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Adam MP, Feldman J, Mirzaa GM, et al., editors. GeneReviews® [Internet]. Seattle (WA): University of Washington, Seattle; 1993-2024.

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Lynch Syndrome

, MD, MS and , PhD.

Author Information and Affiliations

Initial Posting: ; Last Update: February 4, 2021.

Estimated reading time: 58 minutes

Summary

Clinical characteristics.

Lynch syndrome is characterized by an increased risk for colorectal cancer (CRC) and cancers of the endometrium, ovary, stomach, small bowel, urinary tract, biliary tract, brain (usually glioblastoma), skin (sebaceous adenomas, sebaceous carcinomas, and keratoacanthomas), pancreas, and prostate. Cancer risks and age of onset vary depending on the associated gene. Several other cancer types have been reported to occur in individuals with Lynch syndrome (e.g., breast, sarcomas, adrenocortical carcinoma). However, the data are not sufficient to demonstrate that the risk of developing these cancers is increased in individuals with Lynch syndrome.

Diagnosis/testing.

The diagnosis of Lynch syndrome is established in a proband by identification on molecular genetic testing of a germline heterozygous pathogenic variant in MLH1, MSH2, MSH6, or PMS2 or of an EPCAM deletion.

Management.

Treatment of manifestations: Adenomas of colon: complete endoscopic polypectomy with follow-up colonoscopy every one to two years. For colon cancer, segmental or extended colonic resection is indicated depending on clinical scenario and factors such as age. For individuals with rectal adenocarcinoma, proctectomy or total proctocolectomy is indicated. Other tumors are managed as in the general population.

Prevention of primary manifestations: Prophylactic hysterectomy and bilateral salpingo-oophorectomy can be considered after childbearing is completed. Prophylactic colectomy prior to the development of colon cancer is generally not recommended for individuals known to have Lynch syndrome because screening colonoscopy with polypectomy is an effective preventive measure. Aspirin therapy has been shown to decrease the risk for CRC in individuals with Lynch syndrome.

Surveillance: Colonoscopy with removal of precancerous polyps every one to two years beginning between ages 20 and 25 years or two to five years before the earliest CRC diagnosis in the family, whichever is earlier. Annual education for females regarding the symptoms of endometrial and ovarian cancers. Consider transvaginal ultrasound examination and endometrial biopsy every one to two years. Consider upper endoscopy examination every three to five years beginning between ages 30 and 35 years particularly for individuals with a family history of gastric cancer and those of Asian ancestry. Biopsies should be evaluated for H pylori infections so that appropriate treatment can be given as needed. Consider capsule endoscopy and small bowel enterography for distal small bowel cancers. Consider urine analysis with urine cytology to identify microscopic hematuria in those with a family history of urothelial cancer. Consider pancreatic cancer screening in individuals with a family history of pancreatic cancer with alternating endoscopic ultrasound and/or MRI/magnetic resonance cholangiopancreatography.

Agents/circumstances to avoid: High body mass, cigarette smoking, type 2 diabetes, and high cholesterol.

Evaluation of relatives at risk: When a diagnosis of Lynch syndrome has been confirmed in a proband, molecular genetic testing for the Lynch syndrome-related pathogenic variant should be offered to first-degree relatives to identify those who would benefit from early surveillance and intervention. Although molecular genetic testing for Lynch syndrome is generally not recommended for at-risk individuals younger than age 18 years, a history of early cancers in the family may warrant predictive testing prior to age 18.

Genetic counseling.

Lynch syndrome caused by a heterozygous germline pathogenic variant in MLH1, MSH2, MSH6, or PMS2 or by an EPCAM deletion is inherited in an autosomal dominant manner. Individuals with Lynch syndrome caused by constitutional inactivation of MLH1 by methylation typically represent simplex cases but families with non-mendelian inheritance of hypermethylation have been reported. The majority of individuals with Lynch syndrome inherited a pathogenic variant from a parent; however, because of incomplete penetrance, variable age of cancer development, cancer risk reduction as a result of screening or prophylactic surgery, or early death, not all individuals with a pathogenic variant in one of the genes associated with Lynch syndrome have a parent who had cancer. Each child of an individual with Lynch syndrome has a 50% chance of inheriting the pathogenic variant. Prenatal testing for a pregnancy at increased risk is possible if the pathogenic variant in the family is known.

Diagnosis

No consensus clinical diagnostic criteria for Lynch syndrome have been published.

Suggestive Findings

A diagnosis of Lynch syndrome should be suspected in a proband with:

  • A diagnosis of a tumor of the Lynch syndrome spectrum (e.g., colorectal, endometrial, ovarian, stomach, small bowel, urinary tract [urothelial], biliary tract, prostate, brain [usually glioblastoma], skin [sebaceous adenomas, sebaceous carcinomas, and keratoacanthomas], and pancreas) with one of the following on tumor tissue testing:
    • Microsatellite instability (MSI) testing showing that tumor tissue is MSI high. (For information on MSI testing, including advantages and disadvantages, click here.)
    • Immunohistochemistry (IHC) demonstrating loss of expression of one or more of the mismatch repair (MMR) gene products: MLH1, MSH2, MSH6, and/or PMS2. (For information on advantages and disadvantages of IHC testing, click here.)
    • Next-generation sequencing in tumor tissue revealing MSI
    • Identification of a pathogenic variant in tumor tissue in an MMR gene
  • A diagnosis of colorectal cancer (CRC) or endometrial cancer and one or more of the following:*
    • Colorectal or endometrial cancer diagnosed before age 50 years
    • Synchronous or metachronous Lynch syndrome-related cancers (e.g., colorectal, endometrial, ovarian, stomach, small bowel, urinary tract, biliary tract, prostate, brain, sebaceous adenomas, sebaceous carcinomas, keratoacanthomas, pancreatic)
    • Colorectal tumor tissue with MSI-high histology (e.g., poor differentiation, tumor-infiltrating lymphocytes, Crohn-like lymphocytic reaction, mucinous/signet-ring differentiation, medullary growth pattern)
    • At least one first-degree relative with any Lynch syndrome-related cancer diagnosed before age 50 years
    • At least two first-degree relatives with any Lynch syndrome-related cancers regardless of age of cancer diagnosis
  • A family member with colorectal or endometrial cancer who meets one of the above criteria
    Note: Molecular genetic testing ideally begins with a person who has had a Lynch syndrome-related cancer. However, in some families there may be no affected individual who is alive or willing to be tested.
  • A family member with a confirmed diagnosis of Lynch syndrome (pathogenic variant in one of the genes listed in Table 1)
  • A ≥5% probability of having a pathogenic variant in one of the genes listed in Table 1 based on risk assessment models
    Note: Several risk assessment models including PREMM5 [Kastrinos et al 2017], MMRPredict [Barnetson et al 2006], and MMRPro [Chen et al 2006] predict the likelihood of identifying a germline pathogenic variant in one of the genes listed in Table 1. Some data suggest utilizing a lower threshold of ≥2.5% for the PREMM5 predictive model.

* Adapted from revised Bethesda Guidelines and National Comprehensive Cancer Network Guidelines; click here (no-fee registration and login required).

Population screening strategies for Lynch syndrome. Lynch syndrome screening guidelines for individuals have been developed by the NCCN; click here (no-fee registration and login required).

Screening approaches include:

  • Screen all CRC and endometrial cancers with MSI or IHC testing. This was shown to be a cost-effective approach for identifying individuals who should be offered germline molecular genetic testing for Lynch syndrome [EGAPP 2009, Ladabaum et al 2011, Moreira et al 2012, Mange et al 2015]. (For information on universal tumor testing, including advantages and disadvantages of IHC and MSI testing, see Hampel et al [2018].)
  • Use age of onset, familial cancer history, and pathologic features to predict which individuals are more likely to have a germline MMR pathogenic variant [Rabban et al 2014].
  • Tumor tissue sequence analysis for a pathogenic variant in one of the genes listed in Table 1 can simplify the screening and provide additional prognostic and/or treatment information [Hampel et al 2018, Salvador et al 2019]. Note: Simultaneous tumor tissue and germline testing that includes analysis of the genes listed in Table 1 may become the preferred approach because it will (1) simplify the screening protocol, (2) reduce the need for reflex testing, and (3) provide additional prognostic or treatment information [Hampel et al 2018, Salvador et al 2019].

Targeted molecular genetic testing on tumor tissue. Approximately 15% of sporadic CRCs have evidence of MMR deficiency. Determining which CRCs are not due to a Lynch-associated germline pathogenic variant is possible with additional tumor tissue testing on either all CRCs with MSI or on tumors with absence of MLH1/PMS2 on IHC. Targeted tumor tissue testing includes the following:

  • MLH1 promoter methylation analysis. 10%-15% of CRCs are MSI high or MMR deficient due to somatic methylation of the MLH1 promoter silencing gene expression in the tumor tissue.
    Note: Lynch syndrome-related cancers do not have hypermethylation of the MLH1 promoter (see Differential Diagnosis, Sporadic Colorectal Cancer) unless there is constitutional inactivation of MLH1 by promoter methylation.
  • Targeted analysis of BRAF pathogenic variant p.Val600Glu (p.V600E)
    Note: (1) Somatic BRAF pathogenic variant c.1799T>A (p.Val600Glu; NM_004333.4) rarely occurs in colorectal tumor tissue in individuals with Lynch syndrome, while it is present in approximately 15% of all CRCs (see Differential Diagnosis, Sporadic Colorectal Cancer). (2) BRAF pathogenic variants are not common in sporadic endometrial cancers; thus, BRAF testing is not helpful in distinguishing endometrial cancers that are sporadic from those that are Lynch syndrome related. (3) Tumor tissue MLH1 promoter methylation testing is currently considered a more effective screening test for Lynch syndrome than somatic targeted sequence analysis for BRAF p.Val600Glu [Newton et al 2014].

Establishing the Diagnosis

The diagnosis of Lynch syndrome can be established in a proband by identification of a heterozygous germline pathogenic (or likely pathogenic) variant in one of the genes listed in Table 1 using molecular genetic testing.

Note: (1) Per ACMG/AMP variant interpretation guidelines, the terms "pathogenic variants" and "likely pathogenic variants" are synonymous in a clinical setting, meaning that both are considered diagnostic and both can be used for clinical decision making [Richards et al 2015]. Reference to "pathogenic variants" in this section is understood to include any likely pathogenic variants. (2) Identification of a heterozygous variant of uncertain significance in one of the genes listed in Table 1 does not establish or rule out the diagnosis.

Molecular genetic testing approaches can include a multigene panel or DNA methylation studies (see Option 1), and serial single-gene testing (see Option 2). Comprehensive genomic testing (see Option 3) may also be considered.

Option 3

Comprehensive genomic testing (when available) including exome sequencing and genome sequencing may be considered. Such testing may provide or suggest a diagnosis not previously considered (e.g., a pathogenic variant in a different gene or genes that results in a similar clinical presentation). If this option is chosen, it is important that the genes of interest be well covered and the analysis driven by phenotype.

For an introduction to comprehensive genomic testing click here. More detailed information for clinicians ordering genomic testing can be found here.

Table 1.

Molecular Genetic Testing Used in Lynch Syndrome

Gene 1Proportion of Lynch Syndrome Attributed to Pathogenic Variants in Gene 2Proportion of Probands w/a Pathogenic Variant 3 Detectable by Method
Sequence analysis 4, 5, 6Gene-targeted deletion/
duplication analysis 5, 6, 7
MLH1 815%-40%80%-90%10%-20%
MSH2 20%-40%60%-80%20%-40%
MSH6 12%-35%90%-100%0%-10%
PMS2 9, 105%-25%45%-80% 920%-55% 9
EPCAM 11<10%None reported100% 12
1.

See Table A. Genes and Databases for chromosome locus and protein.

2.

Data obtained from universal Lynch syndrome screening for colorectal and endometrial cancers

3.

See Molecular Genetics for information on variants detected in this gene.

4.

Sequence analysis detects variants that are benign, likely benign, of uncertain significance, likely pathogenic, or pathogenic. Variants may include small intragenic deletions/insertions and missense, nonsense, and splice site variants. Detection of exon or whole-gene deletions/duplications require specific sequencing data analysis or use of alternative molecular methods (see footnote 7). For issues to consider in interpretation of sequence analysis results, click here.

5.
6.

Alteration of the proportions may occur in populations with over-representation of specific founder variants.

7.

Gene-targeted deletion/duplication analysis detects intragenic deletions or duplications. Methods used may include specific data analysis of gene panels, quantitative PCR, long-range PCR, multiplex ligation-dependent probe amplification (MLPA), and a gene-targeted microarray designed to detect single-exon deletions or duplications.

8.

Constitutional inactivation of MLH1 by methylation, along with somatic loss of heterozygosity of the functional allele, has been reported to be a rare cause of Lynch syndrome. Such cases are not detectable by either sequence analysis or deletion/duplication analysis of MLH1 (see Molecular Genetics).

9.

Due to the high level of homology between PMS2 and pseudogenes, testing and interpretation of findings in this gene are difficult. A laboratory that adheres to ACMG guidelines for analysis of PMS2 and that has expertise in testing this gene should be selected when a PMS2 pathogenic variant is suspected in a family [Hegde et al 2014]. Long-range PCR, cDNA sequence analysis, and other strategies have been devised to analyze PMS2 [Li et al 2015a, Jansen et al 2020].

10.

Methods to sequence and identify large rearrangements in PMS2 have been developed and improved over time, making it difficult to determine the proportion of pathogenic variants detected by each method in an affected population. Variants detectable by sequence analysis appear to be more common; however, large rearrangements may comprise 20%-50% of pathogenic variants in this gene [van der Klift et al 2010, Vaughn et al 2010, Smith et al 2016, van der Klift et al 2016].

11.

Although EPCAM is not a mismatch repair gene, recurrent germline deletions of the 3' region result in silencing of the adjacent downstream MSH2 by hypermethylation [Niessen et al 2009, Goel et al 2011, Kuiper et al 2011].

12.

Germline deletions of EPCAM result in silencing of the adjacent MSH2 allele by hypermethylation. The adjacent MSH2 allele itself is not mutated (see Molecular Pathogenesis). Sequence analysis of EPCAM without deletion analysis is not appropriate for diagnosis of Lynch syndrome; methods for the detection of large rearrangements should be used (see footnote 7).

Table 2.

Tumor Tissue Test Results, Interpretation, and Additional Testing Options

Tumor Testing 1Plausible EtiologiesAdditional Testing Options for Lynch Syndrome 3, 4, 5
ImmunohistochemistryMSIBRAF V600E 2MLH1 Promoter Methylation
MLH1 MSH2 MSH6 PMS2
++++MSS
  • Sporadic cancer
  • Cancer due to other hereditary cancer syndrome
None 6
++++MSI high
  • Sporadic cancer
  • Germline MMR gene pathogenic variant
  • Germline MMR gene testing or paired germline/tumor tissue MMR gene testing
  • If germline testing negative & paired germline/tumor tissue not done, consider tumor tissue MMR gene testing.
MSI high
  • Sporadic cancer
  • Germline MMR gene pathogenic variant
  • IHC
  • If IHC not available, consider germline MMR gene testing or paired germline/tumor tissue MMR gene testing.
  • If germline testing negative & paired germline/tumor tissue not done, consider tumor tissue MMR gene testing.
++
  • Sporadic cancer
  • Germline MLH1 pathogenic variant
  • Germline PMS2 pathogenic variant (rare)
  • Targeted BRAF &/or MLH1 promoter methylation testing on tumor tissue
  • If BRAF/MLH1 methylation normal, germline MMR gene testing or paired germline/tumor tissue MMR gene testing
  • If germline testing negative & paired germline/tumor tissue not done, consider tumor tissue MMR gene testing.
++Pos
  • Sporadic cancer
  • Germline MLH1 path var (rare)
  • Constitutional MLH1 epimutation
  • If early-onset cancer (< age 50 yrs) or significant family history of cancer: germline MMR gene testing
  • If not: no additional testing
  • For early onset only: constitutional MLH1 epimutation testing 7
++NegPos
  • Sporadic cancer
  • Germline MLH1 path var (rare)
  • Constitutional MLH1 epimutation
++NegNeg
  • Germline MLH1 path var
  • Germline PMS2 path var (rare)
  • Sporadic cancer
  • Germline MMR testing or paired germline/tumor tissue MMR gene testing
  • If germline testing negative & paired germline/tumor tissue not done: consider tumor tissue MMR gene testing.
++
  • Germline MSH2/EPCAM path var
  • Germline MSH6 path var (rare)
  • Sporadic cancer
+++
  • Germline PMS2 path var
  • Germline MLH1 path var
  • Sporadic cancer
+++
  • Germline MSH2/EPCAM path var
  • Sporadic cancer
+++
  • Germline MSH6 path var
  • Germline MSH2/EPCAM path var
  • Sporadic cancer w/treatment effect 8
  • Germline MMR gene testing or germline/tumor tissue MMR gene testing
  • If germline testing negative & paired germline/tumor tissue not done: consider tumor tissue MMR gene testing.
  • If applicable, consider MSI analysis or repeat IHC on nontreated tumor.
+++
  • Sporadic cancer: MLH1 promoter methylation or somatic MLH1 or PMS2 path var
  • Germline MLH1 path var
  • Germline PMS2 path var
  • Targeted BRAF &/or MLH1 promoter methylation testing on tumor tissue
  • If BRAF & MLH1 methylation normal: germline MMR gene testing or paired germline/tumor tissue MMR gene testing
  • If germline testing negative & paired germline/tumor tissue not done: consider tumor tissue MMR gene testing.
  • Germline MMR gene path var
  • Sporadic cancer
  • Targeted BRAF &/or MLH1 promoter methylation testing AND germline MMR gene testing or paired germline/tumor tissue MMR gene testing (often incl MLH1 methylation testing)
  • If germline testing negative & paired germline/tumor tissue not done, consider tumor tissue MMR gene testing

Adapted from Gupta et al [2019].

Empty cells indicate either that testing was not done or that results may not influence testing strategy.

– = absent staining of protein; + = normal staining of protein; IHC = immunohistochemistry; MMR = mismatch repair; MSI = microsatellite instability; MSS = microsatellite stability; Neg = negative; path var = pathogenic variant; Pos = positive

1.

Tumor testing strategies apply to colorectal and endometrial cancers. Limited data exist regarding the efficacy of tumor testing in other types of Lynch syndrome tumors.

2.

BRAF testing is not appropriate for tumors other than colorectal cancer.

3.

45%-68% of tumors with evidence of MMR deficiency have biallelic somatic pathogenic variants. If biallelic somatic pathogenic variants are identified, the affected individual and their relatives should be managed based on the family cancer history and NOT as if they had Lynch syndrome.

4.

Prior to germline genetic testing, proper pre-test counseling should be done.

5.

For information on testing for germline pathogenic variants, see Table 1. A multigene panel that includes MLH1, MSH2, MSH6, PMS2, and EPCAM is recommended. Other colorectal cancer-predisposing genes (e.g., MUTYH, POLE, POLD1, NTHL1) should also be considered (see Differential Diagnosis).

6.

In the presence of a strong family history (e.g., Amsterdam criteria are met), or if additional features of a hereditary cancer syndrome are present, additional testing may be warranted in the proband or tumor testing in another affected family member because of the possibility that the original tumor selected for testing was a sporadic colorectal cancer (phenocopy).

7.

Constitutional MLH1 epimutation testing involves MLH1 promoter hypermethylation analysis on blood or other sources of normal tissue.

8.

Absent MSH6 IHC staining in rectal tumors may be due to treatment effect (neoadjuvant chemoradiotherapy).

Clinical Characteristics

Clinical Description

Individuals with Lynch syndrome are at increased risk for colorectal cancer (CRC) and other cancers including those of the endometrium, ovary, stomach, small bowel, urinary tract, biliary tract, brain (usually glioblastoma), skin (sebaceous adenomas, sebaceous carcinomas, and keratoacanthomas), pancreas, and prostate (Table 3).

Table 3.

Cancer Risks by Gene in Individuals with Lynch Syndrome by Age 70 Years Compared to the General Population

Cancer
Location
General
Population
Risk by Age 74 1
Cancer Risk by Age 70 2, 3
MLH1 MSH2 MSH6 PMS2 EPCAM
FMFMFMF&MF&M
Any20%78%64%77%71%62%28%22%
Colorectum2% 444%53%42%46%20%12%3%75% 5
Endometrium1% 435%46%41%13%12% 5
Ovary0.7%11%17%11%3%
Stomach1%8%16%10%16%2%4%4%
Small bowel<1%
Ureter, kidney<1%3%4%13%16%6%2%
Urinary bladder<1%3%5%7%9%1%4%
Prostate4%7%16%5%5%
Brain<1%2%1%2%4%1%2%
Breast5% 411%13%11%8%

F = female; M = male

1.

Cumulative risk (age: 0-74) for both sexes estimated from worldwide data [Bray et al 2018, Ferlay et al 2018]; see gco​.iarc.fr/today/fact-sheets-cancers for region-specific cancer risks.

2.

Organ-specific cancer risks calculated based on an international multicenter prospective observational study (Prospective Lynch Syndrome Database) using independent test and validation cohorts including 6,350 individuals with class 4 (likely pathogenic) or class 5 (pathogenic) variants and 51,646 follow-up years [Dominguez-Valentin et al 2020]

3.

Data on cancer risks for those with an EPCAM deletion are limited (see Phenotype Correlations by Gene).

4.

Lifetime (birth to death) cumulative cancer risks for colorectal, endometrial, and breast cancers have been estimated to be 4%, 3%, and 13%, respectively, for the US population [Siegel et al 2020].

5.

As of December 2020 there are no data from the Prospective Lynch Syndrome Database for EPCAM. The information included in the table has been obtained from Kempers et al [2011]. The authors observed that risk for CRC is similar to that of MLH1 or MSH2 heterozygotes.

Dowty et al [2013], using sophisticated statistical methodology, revealed that the average risk of cancer (represented in Table 3) does not accurately represent the distribution of cancer risk in individuals with Lynch syndrome. For example, while the average risk of CRC could be 30%-40%, a significant proportion of people with Lynch syndrome have a low risk for CRC (<10%) and a significant proportion have a high risk of developing CRC (>80%). The distribution of cancer risks is due to genetic and/or environmental modifiers.

Colorectal cancer (CRC). The risk of developing CRC associated with MLH1 and MHS2 pathogenic variants is significantly higher than the risk associated with MSH6 or PMS2 pathogenic variants. Of note, risk estimations based on cohort studies compared to the Prospective Lynch Syndrome Database are higher, particularly for PMS2 (9%-20% vs 3%). The mean ages at onset for CRC in individuals with MSH6 and PMS2 pathogenic variants are older than for CRC associated with MLH1 and MSH2 pathogenic variants: 42-69 years for MSH6 and 61-66 years for PMS2, compared with 44 years for MLH1 and MSH2 [Gupta et al 2019, NCCN 2020]. These data explain why CRC screening in individuals with an MLH1 or MSH2 pathogenic variant should start earlier than in individuals with an MSH6 or PMS2 pathogenic variant unless family history suggests otherwise.

CRCs with MSI tend to have a better prognosis in a stage-wise comparison than MSS tumors, potentially reflecting active anti-tumor immune responses. Moreover, treatments supporting the anti-tumoral immune response, such as the immune checkpoint blockade therapy, showed great success in MSI-high tumors [Le et al 2017].

The risk of recurrent CRC is increased in individuals with Lynch syndrome. A meta-analysis of six studies including a total of 871 individuals found that based on an average of 91 months' follow up, the rate of metachronous cancers was 23% among those individuals who had a segmental colectomy, compared to 6% among individuals who had a colectomy (colectomy defined as subtotal or colectomy with ileosigmoid anastomosis) [Anele et al 2017]. The risk of metachronous CRC may be as high as 43% for individuals with an MLH1 or MSH2 pathogenic variant who have segmental resection. Available data indicate that risks of metachronous CRC may be lower for individuals with an MSH6 pathogenic variant, and negligible or absent for those with a PMS2 pathogenic variant.

Endometrial cancer. According to the Prospective Lynch Syndrome Database, the highest risks for endometrial cancer occur in those with MSH2 and MSH6 pathogenic variants (46% and 41% by age 70, respectively), followed by MLH1 (35%), also agreeing with cohort studies [Gupta et al 2019]. In individuals with a PMS2 pathogenic variant, the risk of endometrial cancer is 12%-26%, depending on the study type.

The mean age at endometrial cancer diagnosis is between 47 and 50 years for MLH1, MSH2 and PMS2, and between 53 and 55 years for MSH6. The risk for subsequent endometrial cancer in females with Lynch syndrome presenting first with CRC has been estimated at 26% within ten years of the initial CRC diagnosis [Obermair et al 2010]. As occurs for CRC, endometrial cancers with MSI show better prognosis [Ramchander et al 2020].

Ovarian cancer risk in females with a germline MLH1, MSH2, or MSH6 pathogenic variant has been found to be 11%-17% by age 70. Risk estimates obtained from cohort studies show high variability. Females with a germline PMS2 pathogenic variant have a relatively low increased risk for ovarian cancer. The mean age of diagnosis of Lynch syndrome-associated ovarian cancer has been reported between age 43 and 46 years. Most Lynch syndrome-associated ovarian cancers are of endometrioid histologic subtype [Crosbie et al 2021]. Borderline ovarian tumors do not appear to be associated with Lynch syndrome [Watson et al 2001].

Gastric and small bowel cancers. The risk of gastric and small bowel cancers in individuals with an MLH1 or MSH2 pathogenic variant is 8%-16%. The risk is relatively low for individuals with an MSH6 or PMS2 pathogenic variant. Intestinal-type adenocarcinoma, the most commonly reported pathology of Lynch syndrome-related gastric cancers [Aarnio et al 1997], differs histologically from the diffuse gastric cancer that is most commonly seen in hereditary diffuse gastric cancer, caused by pathogenic variants in CDH1 [Guilford et al 1999]. However, Capelle et al [2010] reported that up to 20% of Lynch syndrome-related gastric cancers may be the diffuse type.

The duodenum and jejunum are the most common sites for cancer of the small bowel, with approximately 50% in reach of upper endoscopy [Schulmann et al 2005]. The majority of small bowel cancers are adenocarcinomas [Rodriguez-Bigas et al 1998, Schulmann et al 2005].

Urinary tract cancers. The urinary tract cancers most commonly associated with Lynch syndrome are transitional carcinomas of the ureter, renal pelvis, and kidney. Bladder cancer risk is also increased in individuals with Lynch syndrome [Dominguez-Valentin et al 2020]. Risk estimates for urinary tract cancers vary significantly based on the individual's sex and the gene involved (see Table 3). Individuals with Lynch syndrome and a prior diagnosis of CRC are also at increased risk for subsequent bladder cancer (7%) and other urinary tract cancers (kidney, renal pelvis, and ureter) (13%) [Win et al 2013].

Prostate cancer. A pathogenic variant in a mismatch repair (MMR) gene was identified in four of 692 men (0.5%) with metastatic prostate cancer [Pritchard et al 2016], and in 26 of 1,501 men (1.7%) with prostate cancer and no prior genetic testing [Pritzlaff et al 2020]. The Prospective Lynch Syndrome Database estimates the risk of prostate cancer for men with an MSH2 pathogenic variant at 16%, and 5%-7% for men with a pathogenic variant in one of the other MMR genes. The mean age at prostate cancer diagnosis was 59-63 years [Gupta et al 2019].

Brain tumors. Data from the National Danish Hereditary Nonpolyposis Colorectal Cancer Register indicated that primary brain tumors were identified in 41 of 288 (14%) Lynch syndrome families, mainly in those with an MSH2 pathogenic variant. Glioblastoma was the most frequent histologic subtype (56%), followed by astrocytoma (22%) and oligodendroglioma (9%) [Therkildsen et al 2015].

Sebaceous neoplasms described in individuals with Lynch syndrome include sebaceous adenomas, sebaceous epitheliomas, sebaceous carcinomas, and keratoacanthomas. Sebaceous neoplasms associated with Lynch syndrome are typically MSI high [Entius et al 2000, Machin et al 2002]. Sebaceous tumors are detected in 1%-9% of individuals with Lynch syndrome, although the available data are limited [Ponti et al 2006, South et al 2008, Ferreira et al 2020].

Pancreatic cancer. Numerous pancreatic cancer cohort studies have identified individuals with a pathogenic variant in an MMR gene [Grant et al 2015, Salo-Mullen et al 2015, Takeuchi et al 2018, Yurgelun et al 2019].

Other Cancers

Breast cancer. The data from the Prospective Lynch Syndrome Database point to a 8%-13% risk by age 70, similar to what is observed in cohort studies [Gupta et al 2019], and representing a marginal increase compared with the general population. To date there is not enough evidence to support additional screening beyond population-based breast cancer screening recommendations or those based on personal/family history of breast cancer.

Additional cancer risks. Several other cancer types have been reported to occur in individuals with Lynch syndrome. In some instances, MSI and/or IHC testing of tumor tissue demonstrated concordance between the extracolonic cancer and the germline pathogenic variant identified in the affected individual. While such findings suggest that the underlying presence of a pathogenic variant in an MMR gene contributed to the development of the cancer, data are not sufficient to demonstrate that the risk of developing these cancers is increased in individuals with Lynch syndrome.

  • Several types of sarcomas have been reported in individuals with an MMR pathogenic variant, including fibrous histiocytomas, rhabdomyosarcomas, leiomyosarcoma, and liposarcoma [Sijmons et al 2000, den Bakker et al 2003, Nilbert et al 2009]. Nilbert et al [2009] determined that six of eight sarcomas in individuals with Lynch syndrome exhibited defective MMR, suggesting that sarcomas may also be part of the spectrum of Lynch syndrome tumors. Due to the rarity of sarcomas it has been difficult to determine the risk associated with Lynch syndrome.
  • Adrenocortical carcinoma (ACC) has also been reported in families with Lynch syndrome. The most extensive study of this association, performed through a hereditary cancer clinic at the University of Michigan, found that two (1.7%) of 114 individuals presenting with ACC had a family history consistent with Lynch syndrome and had a pathogenic variant in an MMR gene identified. This association was further evaluated by case review of 135 individuals with pathogenic variants in an MMR gene, which identified two (1.4%) individuals who also had ACC [Raymond et al 2013].

Lynch Syndrome Variants

Muir-Torre syndrome is an uncommon variant of Lynch syndrome that describes individuals presenting with the combination of sebaceous neoplasms of the skin and one or more visceral malignancies, commonly those seen in Lynch syndrome. The types of sebaceous skin neoplasms described include sebaceous adenomas, sebaceous epitheliomas, sebaceous carcinomas, and keratoacanthomas [John & Schwartz 2016].

Turcot syndrome is a historical term used to describe individuals presenting with CRC or one or more colorectal adenomas in addition to tumors of the central nervous system. Turcot syndrome is usually caused by either a pathogenic variant in one of the MMR genes or an APC pathogenic variant (see APC-Associated Polyposis Conditions). The pathology of the CNS tumor can help distinguish between the underlying genetic causes: APC pathogenic variants are more commonly associated with medulloblastoma; pathogenic variants in MMR genes are more commonly associated with glioblastoma.

Constitutional MMR deficiency (CMMRD) is a rare childhood cancer predisposition syndrome caused by biallelic pathogenic variants in MLH1, MSH2, MSH6, or PMS2. Affected individuals often have CRC or cancer of the small intestine prior to the second decade of life. In a review of 146 individuals with CMMRD, colonic adenomas were the most frequent finding [Wimmer et al 2014]. The cutaneous phenotype in affected individuals may be remarkably similar to that seen in neurofibromatosis type I, as nearly all will have café au lait macules [Wimmer 2012, Bakry et al 2014]. Hematologic cancers and brain tumors have also been reported [Wimmer & Etzler 2008, Durno et al 2010, Bakry et al 2014].

Features in the family history that increase suspicion of CMMRD include a family history of Lynch syndrome, consanguineous parents, and/or at least one parent with clinical findings of Lynch syndrome. However, this diagnosis should not be excluded if the family history is negative, as a significant number of children with CMMRD will not have a family history consistent with Lynch syndrome [Bakry et al 2014]. A European consortium developed clinical criteria indicating when to test for CMMRD [Wimmer et al 2014, Suerink et al 2021].

Phenotype Correlations by Gene

Cancer risks vary among the genes associated with Lynch syndrome (see Table 3).

Germline pathogenic variants in MSH6 and PMS2 are estimated to have lower disease penetrance and older ages at CRC diagnosis [Goodenberger et al 2016, Haraldsdottir et al 2017].

MLH1. Heterozygosity for an MLH1 pathogenic variant is associated with the highest risk for CRC, while the risk for extracolonic cancers is smaller than for MSH2 heterozygotes. MLH1 may also be silenced by constitutional epimutation (MLH1 promoter methylation). In this case, available evidence suggests that constitutional MLH1 epimutations cause a severe Lynch syndrome phenotype, including young age of cancer onset and high risk for multiple primary tumors [Pinto et al 2018].

MSH2. Heterozygosity for an MSH2 pathogenic variant is associated with the greatest risk for extracolonic cancers. MSH2 pathogenic variants have been reported more commonly than a pathogenic variant in the other three MMR genes in individuals with the Muir-Torre variant of Lynch syndrome [Everett et al 2014, Lamba et al 2015, Jessup et al 2016].

MSH6. CRC in individuals with an MSH6 pathogenic variant may be later in onset and more distally located than CRC in individuals with a pathogenic variant in MLH1 or MSH2. Slightly lower risks for CRC and risks for endometrial cancer similar to those of MSH2 heterozygotes have been reported in individuals with an MSH6 pathogenic variant. MSH6-associated cancers may be missed on MSI testing because MSH6 is preferentially involved in the repair of mononucleotide repeats and mononucleotide markers are not included in all MSI panels.

PMS2. Heterozygosity for a PMS2 pathogenic variant is associated with the lowest risk (22%) for any Lynch syndrome-related cancer [Dominguez-Valentin et al 2020]. However, while the overall risk for CRC is lower, age of onset may still be early. A review of 234 individuals with a PMS2 pathogenic variant found that 8% were diagnosed before age 30 [Goodenberger et al 2016].

EPCAM. Deletions of EPCAM that result in epigenetic silencing of MSH2 are associated with a significantly increased risk for CRC. Individuals with an EPCAM deletion typically have early-onset CRC and a CRC cumulative risk up to 75%. Compared to individuals with an MSH2 pathogenic variant, individuals with an EPCAM deletion rarely develop extra-gastrointestinal tumors, including endometrial cancer [Kempers et al 2011].

Genotype-Phenotype Correlations

EPCAM. The risk for extracolonic cancers is dependent on the size of the deletion. 3' EPCAM deletions have been shown to confer a lower risk for extracolonic cancers, whereas deletions that extend into MSH2 confer extracolonic cancer risks similar to intragenic MSH2 pathogenic variants [Tutlewska et al 2013].

Penetrance

Penetrance of CRCs and extracolonic cancers associated with pathogenic variants in an MMR gene or EPCAM is less than 100% (see Table 3). Therefore, some individuals with a cancer-predisposing pathogenic variant in an MMR gene or EPCAM may never develop cancer.

Nomenclature

Lynch syndrome may also be referred to as hereditary non-polyposis colorectal cancer (HNPCC). However, HNPCC currently encompasses Lynch syndrome and all other forms of MMR-deficient and MMR-proficient hereditary nonpolyposis colorectal cancer (even those where a genetic cause has not been identified), whereas the diagnosis of Lynch syndrome requires identification of a pathogenic variant in an MMR gene or EPCAM, or a constitutional MLH1 epimutation.

Prevalence

The population prevalence of Lynch syndrome has been estimated at 1:279 (1 in 1,946 for MLH1, 1 in 2,841 for MSH2, 1 in 758 for MSH6, and 1 in 714 for PMS2) [Win et al 2017]. With the exception of a few founder deletions (see Molecular Genetics), alterations in EPCAM are rare.

Lynch syndrome accounts for approximately 3% of CRCs and 3% of endometrial cancers [Moreira et al 2012, Jiang et al 2019, Kahn et al 2019, Dong et al 2020].

Differential Diagnosis

Hereditary Cancer Syndromes

Table 4.

Hereditary Cancer Syndromes with Increased Risk of Colorectal Cancer in the Differential Diagnosis of Lynch Syndrome

Gene(s)DisorderMOIPolypsColorectal CancerOther Associated Cancers / Clinical Manifestations
RiskMean Age of Onset (Years)
RPS20 RPS20-assoc hereditary nonpolyposis CRC 1ADNoHigh (MMR proficient tumors)AdultNo other assoc cancers / clinical manifestations
APC Familial adenomatous polyposis (FAP) (See APC-Assoc Polyposis Conditions.)ADColonic, gastric & duodenal adenomas (>100 cumulative polyps)~100% if untreated
  • 39 (range: 34-43)
  • Polyp diagnosis: 16 (range: 7-36)
  • CHRPE
  • Osteomas, supernumerary teeth, odontomas
  • Desmoids, epidermoid cysts
  • ↑ risk of medulloblastoma, thyroid papillary carcinoma, hepatoblastoma, & pancreatic, gastric & duodenal cancers
Attenuated familial adenomatous polyposis (AFAP) (See APC-Assoc Polyposis Conditions.)ADColonic, gastric & duodenal adenomas (10-100 cumulative polyps)70% by age 80 yrs50
  • Upper GI findings & thyroid & duodenal cancer risks are similar to FAP.
  • Other extraintestinal manifestations are unusual.
  • Desmoid tumors assoc w/3' APC variants
POLE Polymerase proofreading-assoc polyposis (PPAP) (See OMIM 615083.)ADColonic adenomas (0-100 cumulative polyps)
  • 30%-40% by age 70 yrs 2
  • CRC may develop in absence of polyposis.
  • Note: Most CRCs are MSS; some are MSI high.
50 2
  • ↑ risk of cancers of endometrium, ovary, brain, breast, & other tumor types
  • Adenomas in upper GI tract
POLD1 Polymerase proofreading-assoc polyposis (PPAP) (See OMIM 612591.)ADColonic adenomas (0-100 cumulative polyps)
  • 50%-60% by age 70 yrs 2
  • CRC may develop in absence of polyposis.
  • Note: Most CRCs are MSS; some are MSI high.
35-40 2
  • ↑ risk of cancers of endometrium, ovary, brain, breast, & other tumor types
  • Adenomas in upper GI tract
MUTYH MUTYH polyposis AR
  • Colonic adenomas (10->100 cumulative polyps)
  • Hyperplastic &/or serrated polyps may occur.
  • Duodenal adenomas
  • 43%-63% by age 60 yrs
  • 80%-90% lifetime risk if untreated
  • CRC may develop in absence of polyposis
  • Note: Most CRCs are MSS; a minority are MSI high.
48
  • Duodenal adenomas are common w/↑ risk of duodenal cancer.
  • ↑ risk of ovarian & bladder malignancies
  • Additional features: thyroid nodules, benign adrenal lesions, jawbone cysts, & CHRPE
NTHL1 NTHL1 tumor syndrome AR
  • Colonic adenomas (1-100 cumulative polyps)
  • Hyperplastic &/or serrated polyps may occur.
  • Duodenal adenomas
High lifetime risk61 3
  • High risk of multiple primary tumors
  • ~35%-78% risk of extracolonic cancer by age 60 yrs
  • ↑ risk of breast & endometrial cancers & other tumors types: cervical, urothelial carcinoma of the bladder, meningiomas, unspecified brain tumors, basal cell carcinomas, head & neck squamous cell carcinomas, & hematologic malignancies
MSH3 MSH3-assoc polyposis (OMIM 617100)AR
  • Colonic adenomas (10-100 cumulative polyps)
  • Duodenal adenomas
UnknownAdult 4↑ risk of benign & malignant neoplasia; thyroid adenomas, mammary intraductal papillomas & cysts, gastric cancer, astrocytoma
MLH3 MLH3-assoc polyposis 5ARColonic adenomas (10->100 cumulative polyps)Unknown48-52↑ risk of breast cancer
BMPR1A
SMAD4
Juvenile polyposis syndrome (JPS)ADHamartomatous polyps in GI tract (stomach, small intestine, colon & rectum)~68% by age 60 yrs42
STK11 Peutz-Jeghers syndrome ADPeutz-Jeghers-type hamartomatous polyps in GI tract (esp in small intestine, but also in stomach, colon, & rectum)39%42-46
  • Peutz-Jeghers-type hamartomatous polyps can occur in extraintestinal sites incl renal pelvis, bronchus, gall bladder, nasal passages, urinary bladder, & ureters.
  • Mucocutaneous pigmentation (melanocytic macules)
  • Gonadal tumors
  • ↑ risk of GI cancers, & cancers of the breast, ovary, cervix, endometrium, pancreas, & testis
Duplication upstream of GREM1Hereditary mixed polyposis syndrome (OMIM 601228)ADMultiple polyps of more than 1 histologic type (adenomas, hyperplastic/serrated, & juvenile), &/or individual polyps w/overlapping histologic features (atypical juvenile w/admixed histologic features)↑ CRC risk (unknown estimate)
  • 40s 6
  • Polyp diagnosis: late 20s or later (also reported in adolescence)
Unknown
RNF43 RNF43-assoc serrated polyposis (OMIM 617108)ADColonic serrated polyposis (0->100 cumulative polyps)↑ CRC risk (unknown estimate)AdultNo extracolonic clinical manifestations reported

AD = autosomal dominant; AR = autosomal recessive; CHRPE = congenital hypertrophy of the retinal pigment epithelium; CRC = colorectal cancer; FAP = familial adenomatous polyposis; GI = gastrointestinal; MOI = mode of inheritance; MSI = microsatellite instability; MSS = microstatellite stable

1.
2.

Buchanan et al [2018]. Data should be taken with caution due to the limited number of heterozygotes considered for the estimation of risks.

3.

Grolleman et al [2019]; data obtained from 33 individuals with biallelic NTHL1 pathogenic variants

4.

Adam et al [2016]. Data obtained from four individuals with biallelic MSH3 pathogenic variants. One individual developed CRC at age 55.

5.

Olkinuora et al [2019] identified MLH3 c.3563C>G (p.Ser1188Ter) in three Finnish individuals and one Swedish individual. Experimental data supports founder origin.

6.

Moderate-Risk Colorectal Cancer (CRC) Predisposition

Multigene panels may include testing for genes and/or variants associated with moderate risk of CRC. For many of these variants there are no clear guidelines for the clinical management of heterozygotes. In many cases, the information from testing for variants associated with moderate penetrance does not change the risk management based on family history alone. Variants associated with moderate risk can confer a roughly twofold increased CRC risk – similar to that associated with having a first-degree relative with CRC [Powers et al 2019].

The most prevalent known variants associated with moderate risk for CRC are listed in Table 5 [Yurgelun et al 2017]. Katona et al [2018] defined a counseling framework for these moderate-penetrance variants based on the estimated CRC risk associated with each variant [Ma et al 2014] and the estimated CRC risk for average-risk individuals.

Table 5.

Most Prevalent Known Variants Associated with Moderate Risk for CRC

GenePathogenic VariantCRC Risk 1
APC p.Ile1307Lys 24%
CHEK2 c.1100del3.8%
CHEK2 p.Ile157Thr3.2%
MUTYH 3All germline MUTYH pathogenic variants2.4% 4
1.

Katona et al [2018]; cumulative risk by age 70

2.

Present in ~7% of individuals with Ashkenazi Jewish ancestry. Individuals with this variant do not have polyposis.

3.

Germline heterozygous MUTYH variants are present in ~2% of the general population [Yurgelun et al 2017]; see also MUTYH Polyposis, Individuals Heterozygous for a Germline MUTYH Pathogenic Variant.

4.

The CRC risk estimates for monoallelic MUTYH pathogenic variants are conflicting, and there is no consensus about whether these individuals have increased CRC risk compared to the general population [Ma et al 2014, Katona et al 2018]. The NCCN Panel recommends screening for CRC mainly based on family history. For specific recommendations, see www​.nccn.org (no-fee registration and login required).

Sporadic Colorectal Cancer

Sporadic MMR-deficient tumors commonly occur in older individuals (predominantly in females). These tumors show lack of MLH1 protein expression due to MLH1 promoter methylation and are strongly associated with the CpG island methylator phenotype (CIMP) and the serrated route of carcinogenesis related to somatic activating hotspot oncogenic variants in BRAF.

  • BRAF-related. Somatic BRAF pathogenic variants, the most common being p.Val600Glu (p.V600E) NM_004333.4, occur in 15% of all CRC and, in rare instances, may be identified in tumor tissue from individuals with Lynch syndrome. In a meta-analysis Bläker et al [2020] showed the frequency of BRAF somatic pathogenic variants in Lynch syndrome-associated tumor tissue was 1.6%. The prevalence of BRAF pathogenic variants in MSI-high CRCs also increased with age. Although effective for screening for Lynch syndrome in older age groups, BRAF testing is cost-inefficient for screening in those with MSI-high CRCs diagnosed before age 50 [Bläker et al 2020].
  • Somatic MLH1 promoter methylation. Between 10% and 15% of CRCs are MSI high or MMR deficient due to somatic methylation of the promoter region of MLH1 that silences gene expression in the tumor tissue, rather than due to Lynch syndrome. Sporadic endometrial cancers may also be found to be MSI high or show MMR deficiency due to somatic MLH1 promoter methylation. Tumor MLH1 promoter methylation testing is currently considered a more effective screening test for Lynch syndrome than BRAF p.V600E testing [Newton et al 2014].
    Despite its rarity, analysis for constitutional MLH1 epimutation when MLH1 promoter methylation is identified in a tumor is recommended.
    Individuals in whom a Lynch syndrome-associated germline pathogenic variant is not identified and who have somatic MLH1 promoter methylation are likely to have sporadic cancer. Management and additional surveillance for these individuals should be based on their family history of cancer.

Management

Evaluations Following Initial Diagnosis

To establish the extent of disease and needs in an individual diagnosed with Lynch syndrome, the evaluations summarized in Table 6 are recommended.

Table 6.

Recommended Evaluations Following Initial Diagnosis in Individuals with Lynch Syndrome

System/ConcernEvaluationComment
Colorectal cancer Colonoscopy w/removal of precancerous polyps 1Beginning between ages 20 & 25 yrs or 2-5 yrs before earliest CRC diagnosis in family, whichever is earlier
Endometrial cancer Educate females re symptoms of endometrial cancers (e.g., abnormal uterine bleeding, postmenopausal bleeding).Eval of symptoms should incl endometrial biopsy every 1-2 yrs 2
Screening by endometrial biopsy 2Beginning between ages 30 & 35 yrs
Ovarian cancer Educate females re symptoms assoc w/ovarian cancer (e.g., pelvic or abdominal pain, bloating, ↑ abdominal girth, difficulty eating, early satiety, urinary frequency or urgency).Symptoms that persist for several wks & are a change from baseline should prompt eval by physician.
Gastric & duodenal
cancers
  • Consider upper endoscopy exam esp for those w/family history of gastric cancer & those of Asian ancestry.
  • Biopsies should be evaluated for H pylori infections so that appropriate treatment can be given as needed. 3
Beginning at age 40 yrs
Distal small bowel Consider capsule endoscopy & small bowel enterography.In symptomatic persons
Urinary tract cancers
(renal pelvis, ureter,
&/or bladder)
Consider analysis w/urine cytology to identify microscopic hematuria in those w/family history of urothelial cancer. 4Beginning between ages 30 & 35 yrs
Pancreatic cancer Consider pancreatic cancer screening in carriers w/family history of pancreatic cancer w/alternating EUS &/or MRI/MRCP.Beginning at age 50 yrs 5
Genetic counseling By genetics professionals 6To inform affected persons & their families re nature, MOI, & implications of Lynch syndrome to facilitate medical & personal decision making

CRC = colorectal cancer; EUS = endoscopic ultrasound; MOI = mode of inheritance; MRCP = magnetic resonance cholangiopancreatography

1.

Colonoscopy is recommended rather than flexible sigmoidoscopy because of the predominance of proximal colon cancers in Lynch syndrome.

2.

Studies on the effectiveness of transvaginal ultrasound and endometrial biopsy have not shown them to reduce endometrial cancer mortality. In a systematic review of cost effectiveness of early detection and prevention strategies for endometrial cancer, prophylactic surgery was more effective and less costly than screening with transvaginal ultrasound, CA-125, or endometrial biopsy [Sroczynski et al 2020]. However, in individuals that forgo prophylactic surgery, endometrial cancer surveillance can be performed via endometrial biopsy every 1-2 years [Bercow & Eisenhauer 2019, Gupta et al 2019, NCCN 2020]

3.

Studies have not supported that surveillance for gastric and duodenal cancers improve early detection or outcomes of these cancers, but because the stomach and duodenum are the most common extracolonic non-gynecologic cancer in Lynch syndrome, periodic upper endoscopy exams have been included in guidelines.

4.

There is no clear evidence to support surveillance of urothelial cancers in Lynch syndrome. Surveillance may be considered in selected individuals with a family history of urothelial cancer.

5.

Begin surveillance at 50 years old (or 10 years younger than the earliest exocrine pancreatic cancer diagnosis in the family) for individuals with pancreatic cancer in first- or second-degree relatives from the same side of the family as the identified pathogenic germline variant.

6.

Medical geneticist, certified genetic counselor, or certified advanced genetic nurse

Treatment of Manifestations

Table 7.

Treatment of Manifestations in Individuals with Lynch Syndrome

Manifestation/ConcernTreatment
Adenomas of the colon Complete endoscopic polypectomy w/follow up colonoscopy every 1-2 yrs
Colorectal cancer Segmental or extended colonic resection is indicated depending on clinical scenario & factors such as age. For those w/rectal adenocarcinoma, proctectomy or total proctocolectomy is indicated.
Other tumors Management as in general population

Prevention of Primary Manifestations

Prophylactic hysterectomy and bilateral salpingo-oophorectomy can be considered after childbearing is completed.

Because screening colonoscopy with polypectomy is an effective preventive measure for colorectal cancer, prophylactic colectomy (removal of the colon prior to the development of cancer) is generally not recommended for individuals with Lynch syndrome.

Aspirin therapy has been shown to decrease the risk for CRC in individuals with Lynch syndrome. Based on combined experience, several consensus statements and expert reviews including the NCCN, the Mallorca guidelines, and the US Multi-Society Task Force on CRC suggest that aspirin can be considered, taking into account an individual's personal health and comorbidities, in the management of individuals with Lynch syndrome [Vasen et al 2013, Giardiello et al 2014, Gupta et al 2019]. The CAPP2 study used a dose of 600 mg/day, which is much higher than the dose of 75 mg/day found to be effective for reducing the risk for sporadic CRC. The investigators found that taking 600 mg of aspirin daily for 25 months substantially reduces the risk of CRC (HR=0.42, 95% CI 0.19-0.86; p=0.02) after 55.7 months [Burn et al 2011]. Recently, the investigators reported ten-year follow-up data of the CAPP2 trial. They demonstrated that those taking aspirin had a significantly reduced risk of CRC (HR=0.65, 95% CI 0.43-0.97; p=0.035) as compared to the placebo group [Burn et al 2020]. The CAPP3 study is currently under way with the goal of identifying the minimum dose of aspirin for reducing CRC risk in individuals.

Surveillance

Table 8.

Recommended Surveillance for Individuals with Lynch Syndrome

System/ConcernEvaluationFrequency
Colorectal cancer Colonoscopy w/removal of precancerous polyps 1Every 1-2 yrs beginning between ages 20 & 25 yrs or 2-5 yrs before earliest CRC diagnosis in the family, whichever is earlier
Endometrial
cancer
Educate females re symptoms of endometrial cancers (e.g., abnormal uterine bleeding, postmenopausal bleeding).Annually
Consider transvaginal ultrasound exam & endometrial biopsy 2Every 1-2 yrs
Ovarian cancer Educate females re symptoms assoc w/ovarian cancer (e.g., pelvic or abdominal pain, bloating, ↑ abdominal girth, difficulty eating, early satiety, urinary frequency or urgency).Annually
Gastric &
duodenal cancers
  • Consider upper endoscopy exam esp for those w/family history of gastric cancer & those of Asian ancestry. 3
  • Biopsies should be evaluated for H pylori infections so that appropriate treatment can be given as needed.
Every 3-5 yrs beginning between ages 30 & 35 yrs
Distal small bowel Consider capsule endoscopy & small bowel enterography.In symptomatic persons
Urinary tract
cancers (renal pelvis,
ureter, &/or bladder)
Consider urine analysis w/urine cytology to identify microscopic hematuria in those w/family history of urothelial cancer. 4Annually beginning between ages 30 & 35 yrs
Pancreatic cancer Consider pancreatic cancer screening in those w/family history of pancreatic cancer w/alternating EUS &/or MRI/MRCPAnnually
Other cancers
  • No additional specific screening recommendations for other Lynch syndrome-assoc cancers
  • Follow general population screening guidelines & seek prompt medical attention for changes in health or persistent symptoms.
If there is family history of early onset of other cancer types, cancer screening recommendations should be adjusted to begin screening at an earlier age.

CRC = colorectal cancer; EUS = endoscopic ultrasound; MRCP = magnetic resonance cholangiopancreatography

1.

Colonoscopy is recommended rather than flexible sigmoidoscopy because of the predominance of proximal colon cancers in Lynch syndrome.

2.

Studies on the effectiveness of transvaginal ultrasound and endometrial biopsy have not shown them to reduce endometrial cancer mortality. In a systematic review of cost effectiveness of early detection and prevention strategies for endometrial cancer, prophylactic surgery was more effective and less costly than screening with transvaginal ultrasound, CA-125, or endometrial biopsy [Sroczynski et al 2020]. However, in individuals that forgo prophylactic surgery, endometrial cancer surveillance can be performed via endometrial biopsy every 1-2 years [Bercow & Eisenhauer 2019, Gupta et al 2019].

3.

Upper gastrointestinal endoscopy has recently been recommended for surveillance in individuals with Lynch syndrome [Kumar et al 2020, Ladigan-Badura et al 2021]. However, this has not yet been included in surveillance guidelines for all individuals with Lynch syndrome, rather only in individuals with specific risk factors [see Gupta et al 2019], probably due to the limitations of the published studies, and previous data arguing against the benefit of endoscopic surveillance in Lynch syndrome [Renkonen-Sinisalo et al 2002, Haanstra et al 2015].

4.

Limited data exist to advocate for surveillance for urothelial cancers in Lynch syndrome. Surveillance may be considered in individuals with a family history of urothelial cancer.

Agents/Circumstances to Avoid

There is accumulating evidence that a high body mass, cigarette smoking, type 2 diabetes, and high cholesterol increase the risk of CRC in Lynch syndrome. The direction and strength of observed associations are similar to those for the general population [Win & Scott 2016, Dashti et al 2019].

Evaluation of Relatives at Risk

It is appropriate to clarify the genetic status of all first-degree relatives (parents, sibs, and children) of an affected individual by molecular genetic testing for the Lynch syndrome-related pathogenic variant in the family in order to identify as early as possible those who would benefit from prompt initiation of treatment and preventive measures.

Early recognition of cancers associated with Lynch syndrome may allow for timely intervention and improved final outcome.

  • Sibs should be considered at risk even if the parents have not had cancer because most Lynch syndrome results from an inherited (not de novo) pathogenic variant.
  • If clinical history and family history cannot identify the parent from whom the proband inherited the Lynch syndrome-related pathogenic variant, molecular genetic testing should be offered to both parents to determine which has the pathogenic variant.

In general, molecular genetic testing for Lynch syndrome is not recommended for at-risk individuals younger than age 18 years. However, predictive testing should be considered if there is a history of early-onset cancer in the family. For unaffected individuals with a Lynch syndrome-related pathogenic variant, screening should begin between ages 20 and 25 years, or two to five years earlier than the earliest diagnosis in the family [Gupta et al 2019]. Therefore, a history of early cancers in the family may also warrant testing prior to age 18.

See Genetic Counseling for issues related to testing of at-risk relatives for genetic counseling purposes.

Pregnancy Management

Ideally cancer screening exams would be planned around a pregnancy. An affected female would be encouraged to be current on her cancer screening before attempting to become pregnant. If an affected female is diagnosed with cancer during pregnancy, she should be counseled about cancer treatment options and their potential implications for the fetus.

Therapies Under Investigation

Chromoendoscopy vs narrow band imaging (NBI) vs high-definition white-light colonoscopy for Lynch syndrome surveillance. Two studies compared different colonoscopy imaging modalities against chromoendoscopy. In a study of 138 individuals with Lynch syndrome undergoing back-to-back colonoscopies (first with NBI followed by indigo carmine chromoendoscopy), the adenoma detection rate (ADR) for NBI alone was 20.3% while the ADR for both was 30.4%. A 10.1% difference in detection failed to reach the prespecified noninferiority assumption margin of 5% [Cellier et al 2019]. In another study of 256 individuals with Lynch syndrome randomized to indigo carmine chromoendoscopy versus high-definition white-light colonoscopy, no significant difference in ADR was detected by pancolonic chromoendoscpy (34.4%; 95% CI 26.4%-43.4%) as compared to white-light endoscopy (28.1%; 95% CI 21.1%-36.4%; p=0.28) [Rivero-Sánchez et al 2020]. In both studies, chromoendoscopy better identified flat or diminutive adenomas, but also reported significantly longer withdrawal time with chromoendoscopy.

Oral contraceptives and endometrial cancer risk. Epidemiologic studies have found that use of oral contraceptives for more than one year is associated with significant reduction in endometrial cancer risk (HR 0.39, 95% CI 0.23-0.64) [Dashti et al 2015]. To date there are no prospective trials evaluating the impact of oral contraceptives on endometrial cancer risk. One study has demonstrated reduced endometrial proliferation in women with Lynch syndrome after a three-month course of oral contraceptives [Lu et al 2013]. At this time oral contraceptives are not included in recommendations for women with Lynch syndrome, but they are commonly used for managing routine gynecologic issues and for family planning. Data support that oral contraceptives will likely confer benefits to women with Lynch syndrome similar to those in the general population.

Immunotherapy for Lynch syndrome associated cancers. The development of antibodies to immune checkpoint proteins (anti-PD-1 and anti-CTLA4) demonstrate prolonged T-cell response against cancer cells. The emergence of immune checkpoint inhibitors that manipulate and leverage the immune system represent a breakthrough in treatment of Lynch syndrome-associated (and other MSI-high/MMR-deficient) cancers. Recent studies of the treatment of metastatic MSI-high Lynch associated cancer, not limited to colon cancer, with anti-PD-1 monoclonal antibodies have demonstrated 70% or greater disease control rates [Le et al 2015, Le et al 2017, Overman et al 2017].

Search ClinicalTrials.gov in the US and EU Clinical Trials Register in Europe for access to information on clinical studies for a wide range of diseases and conditions.

Genetic Counseling

Genetic counseling is the process of providing individuals and families with information on the nature, mode(s) of inheritance, and implications of genetic disorders to help them make informed medical and personal decisions. The following section deals with genetic risk assessment and the use of family history and genetic testing to clarify genetic status for family members; it is not meant to address all personal, cultural, or ethical issues that may arise or to substitute for consultation with a genetics professional. —ED.

Mode of Inheritance

In most individuals, Lynch syndrome is caused by a heterozygous germline pathogenic variant in MLH1, MSH2, MSH6, PMS2, or EPCAM, and is inherited in an autosomal dominant manner.

Individuals with Lynch syndrome caused by constitutional inactivation of MLH1 by methylation typically represent simplex cases (i.e., a single occurrence in a family) but families with non-mendelian inheritance of hypermethylation have been reported [Hitchins et al 2011, Hitchins 2015].

Note: Several factors (in addition to the possibility of a constitutional MLH1 epimutation) can hinder the diagnosis of Lynch syndrome based on family history. Screening and removal of precancerous polyps and prophylactic surgery may prevent colon or endometrial cancer in some at-risk relatives; some who died young from other causes may never have developed cancer.

Risk to Family Members

Parents of a proband

  • The majority of individuals diagnosed with Lynch syndrome inherited a pathogenic variant from a parent who may or may not have had cancer.
  • If clinical and family history cannot identify the parent from whom the proband inherited the pathogenic variant, molecular genetic testing should be offered to both parents to determine which parent is heterozygous for the pathogenic variant identified in the proband.
  • In the rare event that the pathogenic variant found in the proband cannot be detected in the leukocyte DNA of either parent (and parental identity testing has confirmed biological maternity and paternity), possible explanations include the following:
    • A de novo pathogenic variant in the proband (The precise de novo pathogenic variant rate for Lynch syndrome is unknown but estimated to be extremely low [Win et al 2011].)
    • Germline mosaicism in a parent (Though theoretically possible, no instances of a proband inheriting a Lynch syndrome-related pathogenic variant from a parent with germline mosaicism have been reported to date.)
  • A parent who is heterozygous for a Lynch syndrome-related pathogenic variant may not have had cancer because of incomplete penetrance, variable age of cancer development, cancer risk reduction resulting from screening or prophylactic surgery, or early death. Therefore, an apparently negative family history cannot be confirmed without appropriate molecular genetic testing to establish that neither parent is heterozygous for the pathogenic variant identified in the proband.

Sibs of a proband. The risk to the sibs of the proband depends on the genetic status of the proband's parents:

  • If a parent of the proband has the pathogenic variant identified in the proband, the risk to the sibs is 50%. Note: Molecular genetic testing for the familial Lynch syndrome-related variant should be offered to all sibs (see Evaluation of Relatives at Risk).
  • If the proband has a known Lynch syndrome-related pathogenic variant that cannot be detected in the leukocyte DNA of either parent, the recurrence risk to sibs is estimated to be 1% because of the theoretic possibility of parental germline mosaicism [Rahbari et al 2016].
  • If the genetic status of the parents is unknown, sibs should be considered at risk for cancers associated with Lynch syndrome (regardless of whether parents have had cancer) and offered molecular genetic testing.

Offspring of a proband. Each child of an individual with Lynch syndrome has a 50% chance of inheriting the Lynch syndrome-related pathogenic variant.

Other family members. The risk to other family members depends on the genetic status of the proband's parents: if a parent has the pathogenic variant (as is the case in most families), the parent's family members are at risk (family history or molecular genetic testing can help determine whether maternal or paternal relatives are at risk).

Related Genetic Counseling Issues

See Management, Evaluation of Relatives at Risk for information on evaluating at-risk relatives for the purpose of early diagnosis and treatment.

Family planning

  • The optimal time for determination of genetic risk and discussion of the availability of prenatal/preimplantation genetic testing is before pregnancy.
  • It is appropriate to offer genetic counseling (including discussion of potential risks to offspring and reproductive options) to young adults who are affected or at risk.

Genetic cancer risk assessment and counseling. For a comprehensive description of the medical, psychosocial, and ethical ramifications of identifying at-risk individuals through cancer risk assessment with or without molecular genetic testing, see Cancer Genetics Risk Assessment and Counseling – for health professionals (part of PDQ®, National Cancer Institute).

Predictive testing (i.e., testing of asymptomatic at-risk individuals)

  • Predictive testing for at-risk relatives is possible once the Lynch syndrome-related pathogenic variant has been identified in an affected family member.
  • Potential consequences of such testing (including but not limited to socioeconomic changes and the need for long-term follow up and evaluation arrangements for individuals with a positive test result) as well as the capabilities and limitations of predictive testing should be discussed in the context of formal genetic counseling prior to testing.

Predictive testing in minors (i.e., testing of asymptomatic at-risk individuals age <18 years)

  • In general, genetic testing for Lynch syndrome is not recommended for at-risk individuals younger than age 18 years. However, predictive testing should be considered if there is a history of early-onset cancer in the family. In unaffected individuals with a Lynch syndrome-related pathogenic variant, screening is recommended beginning at age 20 to 25 years, or two to five years prior to the earliest diagnosis in the family [Gupta et al 2019, NCCN 2020]. Therefore, a history of early cancers in the family may also warrant testing prior to age 18.
  • For more information, see the National Society of Genetic Counselors position statement on genetic testing of minors for adult-onset conditions and the American Academy of Pediatrics and American College of Medical Genetics and Genomics policy statement: ethical and policy issues in genetic testing and screening of children.

In a family with an established diagnosis of Lynch syndrome, it is appropriate to consider testing of symptomatic individuals regardless of age.

Prenatal Testing and Preimplantation Genetic Testing

Once a germline heterozygous Lynch syndrome-related pathogenic variant has been identified in an affected family member, prenatal and preimplantation genetic testing are possible.

Differences in perspective may exist among medical professionals and within families regarding the use of prenatal testing. While most centers would consider use of prenatal testing to be a personal decision, discussion of these issues may be helpful.

Resources

GeneReviews staff has selected the following disease-specific and/or umbrella support organizations and/or registries for the benefit of individuals with this disorder and their families. GeneReviews is not responsible for the information provided by other organizations. For information on selection criteria, click here.

Molecular Genetics

Information in the Molecular Genetics and OMIM tables may differ from that elsewhere in the GeneReview: tables may contain more recent information. —ED.

Table B.

OMIM Entries for Lynch Syndrome (View All in OMIM)

114500COLORECTAL CANCER; CRC
120435LYNCH SYNDROME 1; LYNCH1
120436DNA MISMATCH REPAIR PROTEIN MLH1; MLH1
158320MUIR-TORRE SYNDROME; MRTES
185535EPITHELIAL CELLULAR ADHESION MOLECULE; EPCAM
276300MISMATCH REPAIR CANCER SYNDROME 1; MMRCS1
600259PMS1 HOMOLOG 2, MISMATCH REPAIR SYSTEM COMPONENT; PMS2
600678MutS HOMOLOG 6; MSH6
609309MutS HOMOLOG 2; MSH2
609310LYNCH SYNDROME 2; LYNCH2
613244LYNCH SYNDROME 8; LYNCH8

Molecular Pathogenesis

Lynch syndrome is caused by pathogenic variants in genes involved with the mismatch repair (MMR) pathway. This pathway functions to identify and remove single-nucleotide mismatches or insertions and deletion loops. Pathogenic variants in four of the MMR genes can cause Lynch syndrome [Peltomäki 2003]. The functions of the MMR genes can be disrupted by missense variants, truncating variants, splice site variants, large deletions, or genomic rearrangements. In addition, germline deletions within EPCAM, which is not an MMR gene, can disrupt the MMR pathway by inactivating the adjacent MMR gene MSH2, even though MSH2 itself has not been mutated.

Mechanism of disease causation. Loss of function

Table 9.

Lynch Syndrome: Gene-Specific Laboratory Considerations

Gene 1Special Consideration
EPCAM Only large deletions that incl the last exon of EPCAM are causative of Lynch syndrome; other EPCAM variants are not assoc w/Lynch syndrome [Arnold et al 2020].
MLH1 Constitutional inactivation of the MLH1 promoter by methylation, along w/somatic loss of heterozygosity of the functional allele, has been reported as a rare cause of Lynch syndrome. Most instances of MLH1 promoter methylation are simplex (i.e., a single occurrence in a family), but a few families w/inherited hypermethylation have been reported [Hitchins 2015]. MLH1 promoter methylation is not detectable by either sequence analysis or duplication/deletion analysis of MLH1.
PMS2 Molecular analysis of PMS2 is more complex due to the presence of multiple PMS2 pseudogenes. The presence of genomic regions w/high sequence homology to PMS2 hampers conventional analysis. Long-range PCR, cDNA sequencing, or specific solutions to NGS testing can help distinguish between PMS2 pathogenic variants & pseudogene variants [Li et al 2015a, Lee et al 2021].
1.

Genes in alphabetic order

Notable variants by gene. Table 10 includes founder and common pathogenic variants in different populations.

Table 10.

Lynch Syndrome: Notable Pathogenic Variants by Gene

Gene 1Reference SequencesDNA Nucleotide ChangePredicted Protein ChangeComment / Population 2
EPCAM NM_002354​.2 c.859-1462_*1999del4909
(del exons 8-9)
--Netherlands
c.858+2478_*4507del8674
(del exons 8-9)
--
c.858+2568_*4596del8673
(del exons 8-9)
--Spain
c.858+2488_*7469del11626
(del exons 8-9)
--
c.859-1860_*25547del
(EPCAM del exons 8-9 & MSH2 del exons 1-3)
--
c.859–1430_*2033del
(del exons 8-9)
--Italy
MLH1 NM_000249​.3
NP_000240​.1
c.1731+2247_1897-402del
(del exon 16)
p.Pro579_Glu633delFinland
NM_000249​.3 c.454-1G>A--
NM_000249​.3
NP_000240​.1
c.112A>Cp.Asn38HisNetherlands
NM_000249​.3 c.306+5G>A--Spain; variants are assoc w/moderate penetrance.
NM_000249​.3
NP_000240​.1
c.1865T>Ap.Leu622His
NM_000249​.3 c.1896+280_*8935del11626
(MLH1 del exons 17-19 & LRRFIP2 del exons 26-29)
--Portugal
c.545+3A>G--Italy, Canada-Quebec (persons of Italian ancestry) & Brazil
c.589-2A>G--United States & Italy
NM_000249​.3
NP_000240​.1
c.731G>Ap.Gly244AspItaly
NM_000249​.3 c.1558+1G>T--
NM_000249​.3
NP_000240​.1
c.2252_2253delAAp.Lys751SerfsTer3
c.2269dupTp.(*757LeuextTer33)
c.1731G>Ap.Ser556ArgfsTer14
c.1489dupCp.Arg497ProfsTer6Germany
NM_000249​.3 c.1667+2_1667+8delTAAATCAinsATTTDenmark
NM_000249​.3
NP_000240​.1
c.2142G>Ap.Trp714TerSwitzerland
c.2195_2198dupAACAp.His733GlnfsTer14Canada-Quebec
c.1831_1832delATp.Ile611CysfsTer2
c.1039-2329_1409+827del3527p.Thr347LysfsTer8
c.1381A>Tp.Lys461TerUnited States
c.2044_2045delATp.Met682ValfsTer11Puerto Rico
c.392C>Gp.Ser131TerRepublic of Macedonia
NM_000249​.3 1.8-kb deletion of exon 11--China
NM_000249​.3
NP_000240​.1
c.793C>Tp.Arg265CysTaiwan
c.1758dupCp.Met587HisfsTer6Korea
MSH2 NM_000251​.2 c.942+3A>T--Common worldwide
NM_000251​.2
NP_000242​.1
c.388_389delCAp.Gln130ValfsTer2Portugal, South America
c.2152C>Tp.Gln718TerPortugal
c.2063T>Gp.Met688ArgSpain
NM_000251​.2 c.[2635-3C>T; 2635-5T>C]--
c.-3568_*28336del36681
(del exons 4-8)
--
c.*4136_*13502del9366
(del exon 7)
--
c.-11844_1077-6021delins(155)
(del exons 1-6)
--Italy
c.1277−1180_1386+2226del3516insCATTCTCTTTGAAAA)
(del exon 8)
--
c.1276+198_1386+3761del19280
(del exon 8)
--
NM_000251​.2
NP_000242​.1
c.1786_1788delAATp.Asn596delDenmark
NM_000251​.2 c.-823_1076+5984del
(del exons 1-6)
United States
NM_000251​.2
NP_000242​.1
c.1906G>Cp.Ala636ProAshkenazi Jews
c.1165C>Tp.Arg389TerCanada-Quebec
c.2185_2192delATGTTGGAinsCCCTp.Met729ProfsTer2Chile
c.1457_1460delATGAp.Asn486fsTer10China (Guangdong)
MSH6 NM_000179​.2
NP_000170​.1
c.467C>Gp.Ser156TerNetherlands
c.651dupTp.Lys218Ter
c.1614_1615delTCinsAGp.Tyr538Ter
c.2983G>Tp.Glu995TerFinland
c.1346T>Cp.Leu449ProSweden
c.2931C>Gp.Tyr977Ter
c.3959_3962delCAAGp.Ala1320GlufsTer6Ashkenazi Jews
c.3984_3987dupGTCAp.Leu1330ValfsTer12
PMS2 NM_000535​.6 c.989-1G>T--Norway
NM_000535​.6
NP_000526​.2
c.736_741delCCCCCTins11p.Pro246CysfsTer3United States
c.137G>Tp.Ser46IleUnited States
c.1A>Gp.Met1?
c.903G>Tp.Lys301Asn
c.989-296_1144+706del1158
(del exon 10)
p.Glu330_Glu381delAustralia
c.2002A>Gp.Ile668ValInuit

Variants listed in the table have been provided by the authors. GeneReviews staff have not independently verified the classification of variants.

GeneReviews follows the standard naming conventions of the Human Genome Variation Society (varnomen​.hgvs.org). See Quick Reference for an explanation of nomenclature.

1.

Genes from Table 1 in alphabetic order

2.

Chapter Notes

Author History

Stephen B Gruber, MD, PhD; USC Norris Comprehensive Cancer Center (2004-2021)
Gregory Idos, MD, MS (2021-present)
Wendy Kohlmann, MS; University of Utah Huntsman Cancer Institute (2004-2021)
Laura Valle, PhD (2021-present)

Revision History

  • 4 February 2021 (sw) Comprehensive update posted live
  • 12 April 2018 (sw) Revision: Tumor testing table added (Table 2)
  • 1 February 2018 (sw) Comprehensive update posted live
  • 22 May 2014 (me) Comprehensive update posted live
  • 20 September 2012 (cd) Revision: Multigene panels for Lynch syndrome (hereditary non-polyposis colon cancer) available clinically
  • 11 August 2011 (me) Comprehensive update posted live
  • 29 November 2006 (me) Comprehensive update posted live
  • 5 February 2004 (me) Review posted live
  • 18 April 2003 (sg) Original submission

References

Published Guidelines / Consensus Statements

  • American College of Medical Genetics technical standards and guidelines for genetic testing for inherited colorectal cancer (Lynch syndrome, familial adenomatous polyposis, and MYH-associated polyposis). Available online. 2014. Accessed 5-11-23.
  • American College of Medical Genetics/American Society of Human Genetics. Joint statement on genetic testing for colon cancer (pdf). Available online. 2000. Accessed 5-11-23.
  • American Gastroenterological Association. Medical position statement: hereditary colorectal cancer and genetic testing (pdf). Available online. 2001. Accessed 5-11-23.
  • American Society of Clinical Oncology. Policy statement update: genetic testing for cancer susceptibility. Available online. 2010. Accessed 5-11-23.
  • American Society of Colon and Rectal Surgeons. Practice parameters for the treatment of patients with dominantly inherited colorectal cancer (FAP and HNPCC). Available online. 2003. Accessed 5-11-23.
  • Committee on Bioethics, Committee on Genetics, and American College of Medical Genetics and Genomics Social, Ethical, Legal Issues Committee. Ethical and policy issues in genetic testing and screening of children. Available online. 2013. Accessed 5-11-23.
  • Giardiello FM, Brensinger JD, Petersen GM. American Gastroenterological Association technical review on hereditary colorectal cancer and genetic testing. Gastroenterology. 2001;121:198-213. [PubMed]
  • Lu KH, Wood ME, Daniels M, Burke C, Ford J, Kauff ND, Kohlmann W, Lindor NM, Mulvey TM, Robinson L, Rubinstein WS, Stoffel EM, Snyder C, Syngal S, Merrill JK, Wollins DS, Hughes KS, et al. American Society of Clinical Oncology Expert Statement: collection and use of a cancer family history for oncology providers. J Clin Oncol. 2014;32:833-40. [PubMed]
  • National Comprehensive Cancer Network. Genetic/familial high-risk assessment: colorectal cancer. 2020.
  • National Society of Genetic Counselors. Position statement on genetic testing of minors for adult-onset conditions. Available online. 2018. Accessed 5-11-23.
  • Weissman SM, Burt R, Church J, Erdman S, Hampel H, Holter S, Jasperson K, Kalady MF, Haidle JL, Lynch HT, Palaniappan S, Wise PE, Senter L. Identification of individuals at risk for Lynch syndrome using targeted evaluations and genetic testing: National Society of Genetic Counselors and the Collaborative Group of the Americas on Inherited Colorectal Cancer joint practice guideline. J Genet Couns. 2012;21:484-93. [PubMed]

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