Medicine (RMH) - Research Publications

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Author: Buchanan, Daniel × End date: 2019 ×

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    Clinico-pathological predictors of mismatch repair deficiency in sebaceous neoplasia: A large case series from a single Australian private pathology service
    Walsh, MD ; Jayasekara, H ; Huang, A ; Winship, IM ; Buchanan, DD (WILEY, 2019-05)
    BACKGROUND/OBJECTIVES: Loss of expression of mismatch repair (MMR) proteins is frequently observed in sebaceous skin lesions and can be a herald for Lynch syndrome. The aim of this study was to identify clinico-pathological predictors of MMR deficiency in sebaceous neoplasia that could aid dermatologists and pathologists in determining which sebaceous lesions should undergo MMR immunohistochemistry (IHC). METHODS: An audit of sebaceous skin lesions (excluding hyperplasia) where pathologist-initiated MMR IHC was performed between January 2009 to December 2016 was undertaken from a single pathology practice identifying 928 lesions from 882 individuals. Lesions were further analysed for differences in gender, age at diagnosis, lesion type and anatomic location, stratified by MMR status. RESULTS: The 882 individuals (67.7% male) had a mean (SD) age of diagnosis of 68.4 ± 13.3 years. Nearly two-thirds of the lesions were sebaceous adenomas, with 82.6% of all lesions occurring on the head and neck. MMR deficiency, observed in 282 of the 919 lesions (30.7%), was most common in sebaceous adenomas (210/282; 74.5%). MMR-deficient lesions occurred predominantly on the trunk or limbs (64.7%), compared with 23.2% in head or neck (P < 0.001). Loss of MSH2 and MSH6 protein expression was most frequent pattern of loss (187/281; 66.5%). The highest AUC for discriminating MMR-deficient sebaceous lesions from MMR-proficient lesions was observed for the ROC curve based on subgroups defined by type and anatomic location of the sebaceous lesion (AUC = 0.68). CONCLUSION: The best combination of measured clinico-pathological features achieved only modest positive predictive values, sensitivity and specificity for identifying MMR-deficient sebaceous skin lesions.
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    Current mismatch repair deficiency tumor testing practices and capabilities: A survey of Australian pathology providers
    Mascarenhas, L ; Shanley, S ; Mitchell, G ; Spurdle, AB ; Macrae, F ; Pachter, N ; Buchanan, DD ; Ward, RL ; Fox, S ; Duxbury, E ; Driessen, R ; Boussioutas, A (WILEY, 2018-12)
    AIM & METHODS: An electronic survey of the Royal College of Pathologists of Australasia accredited pathology services was conducted to assess Lynch syndrome tumor screening practices and to identify barriers and capabilities to screen newly diagnosed colorectal and endometrial tumors in Australia. RESULTS: Australia lacks a national policy for universal mismatch repair-deficient (dMMR) testing of incident colorectal and endometrial tumors cases. Routine Lynch syndrome tumor screening program for colorectal and/or endometrial tumors was applied by 95% (37/39) of laboratories. Tumor dMMR screening methods varied; MMR protein immunohistochemistry (IHC) alone was undertaken by 77% of 39 laboratories, 18% performed both IHC and microsatellite instability testing, 5% did not have the capacity to perform in-house testing. For colorectal tumors, 47% (17/36) reported following a universal approach without age limit, 30% (11/36) tested only "red flag" cases; 6% (3/36) on clinician request only. For endometrial tumors, 37% (12/33) reported clinician request generated testing, 27% (9/33) were screening only "red flag" cases, and 12% (4/33) carried out universal screening without an age criteria. BRAF V600E mutation testing of colorectal tumors demonstrating aberrant MLH1 protein expression by IHC was the most common secondary tumor test, with 53% of laboratories performing the test; 15% of laboratories also applied the BRAF V600E test to endometrial tumors with aberrant MLH1 expression despite no evidence for its utility. Tumor testing for MLH1 promoter methylation was performed by less than 15% laboratories. CONCLUSION: Although use of tumor screening for evidence of dMMR is widely available, protocols for its use in Australia vary widely. This national survey provides a snapshot of the current availability and practice of tumor dMMR screening and identifies the need for a uniform national testing policy.
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    Utility of immunohistochemistry for mismatch repair proteins on colorectal polyps in the familial cancer clinic
    Dow, E ; Buchanan, DD ; Winship, IM (WILEY, 2018-11)
    BACKGROUND: Immunohistochemistry for loss of expression of one or more of the mismatch repair proteins is performed on colorectal cancer tissue as a screening test for Lynch syndrome; however, its role in pre-malignant polyps remains controversial. AIM: To determine the effectiveness of mismatch repair immunohistochemistry performed on pre-malignant colorectal polyps in identifying Lynch syndrome, focusing on clinical utility and value. METHODS: A retrospective audit was conducted of mismatch repair immunohistochemistry performed on non-malignant polyps in patients who attended the Family Cancer Clinic at the Royal Melbourne Hospital. Two hundred and six patient records over a 10-year period (2006-2016) were reviewed. Personal and family history data were collected, including genetic testing results. RESULTS: Of the 57 patients who underwent polyp testing, the family histories comprised Amsterdam II Criteria (12.3%), Lynch syndrome-associated malignancies (42.1%), Lynch syndrome-associated malignancies and polyps (35.1%) and polyps only (8.8%); 10.5% of patients had no significant family history. Normal expression of the mismatch repair proteins was observed in 94.7% of patients; loss of expression was observed in three individuals with concordant germline variants in two patients (one PMS2 variant of unknown significance and one MSH6 mutation). Additional genetic testing in 21 patients with normal immunohistochemistry did not identify any additional Lynch syndrome cases. CONCLUSION: The clinical utility of mismatch repair immunohistochemistry on polyp tissue was low. No additional cases of Lynch syndrome were identified, and a large proportion of patients proceeded to germline testing despite normal polyp immunohistochemistry. We suggest there is no value in this approach.
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    Linkage to chromosome 2q32.2-q33.3 in familial serrated neoplasia (Jass syndrome)
    Roberts, A ; Nancarrow, D ; Clendenning, M ; Buchanan, DD ; Jenkins, MA ; Duggan, D ; Taverna, D ; McKeone, D ; Walters, R ; Walsh, MD ; Young, BW ; Jass, JR ; Rosty, C ; Gattas, M ; Pelzer, E ; Hopper, JL ; Goldblatt, J ; George, J ; Suthers, GK ; Phillips, K ; Parry, S ; Woodall, S ; Arnold, J ; Tucker, K ; Muir, A ; Drini, M ; Macrae, F ; Newcomb, P ; Potter, JD ; Pavluk, E ; Lindblom, A ; Young, JP (SPRINGER, 2011-06)
    Causative genetic variants have to date been identified for only a small proportion of familial colorectal cancer (CRC). While conditions such as Familial Adenomatous Polyposis and Lynch syndrome have well defined genetic causes, the search for variants underlying the remainder of familial CRC is plagued by genetic heterogeneity. The recent identification of families with a heritable predisposition to malignancies arising through the serrated pathway (familial serrated neoplasia or Jass syndrome) provides an opportunity to study a subset of familial CRC in which heterogeneity may be greatly reduced. A genome-wide linkage screen was performed on a large family displaying a dominantly-inherited predisposition to serrated neoplasia genotyped using the Affymetrix GeneChip Human Mapping 10 K SNP Array. Parametric and nonparametric analyses were performed and resulting regions of interest, as well as previously reported CRC susceptibility loci at 3q22, 7q31 and 9q22, were followed up by finemapping in 10 serrated neoplasia families. Genome-wide linkage analysis revealed regions of interest at 2p25.2-p25.1, 2q24.3-q37.1 and 8p21.2-q12.1. Finemapping linkage and haplotype analyses identified 2q32.2-q33.3 as the region most likely to harbour linkage, with heterogeneity logarithm of the odds (HLOD) 2.09 and nonparametric linkage (NPL) score 2.36 (P = 0.004). Five primary candidate genes (CFLAR, CASP10, CASP8, FZD7 and BMPR2) were sequenced and no segregating variants identified. There was no evidence of linkage to previously reported loci on chromosomes 3, 7 and 9.
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    Genomic Characterization of Upper-Tract Urothelial Carcinoma in Patients With Lynch Syndrome
    Donahue, TE ; Bagrodia, A ; Audenet, F ; Donoghue, MTA ; Cha, EK ; Sfakianos, JP ; Sperling, D ; Al-Ahmadie, H ; Clendenning, M ; Rosty, C ; Buchanan, DD ; Jenkins, M ; Hopper, J ; Winship, I ; Templeton, AS ; Walsh, MF ; Stadler, ZK ; Iyer, G ; Taylor, B ; Coleman, J ; Lindor, NM ; Solit, DB ; Bochner, BH (AMER SOC CLINICAL ONCOLOGY, 2018-01-23)
    PURPOSE: Patients with Lynch syndrome (LS) have a significantly increased risk of developing upper-tract urothelial carcinoma (UTUC). Here, we sought to identify differences in the patterns of mutational changes in LS-associated versus sporadic UTUCs. PATIENTS AND METHODS: We performed targeted sequencing of 17 UTUCs from patients with documented LS-associated germline mutations (LS-UTUCs) using the Memorial Sloan Kettering Integrated Molecular Profiling of Actionable Cancer Targets targeted exon capture assay and compared the results with those from a recently characterized cohort of 82 patients with sporadic UTUC. RESULTS: Patients with LS-UTUC were significantly younger, had had less exposure to tobacco, and more often presented with a ureteral primary site compared with patients with sporadic UTUC. The median number of mutations per tumor was significantly greater in LS-UTUC tumors than in tumors from the sporadic cohort (58; interquartile range [IQR], 47-101 v 6; IQR, 4-10; P < .001), as was the MSIsensor score (median, 25.1; IQR, 17.9-31.2 v 0.03; IQR, 0-0.44; P < .001). Differences in the genetic landscape were observed between sporadic and LS-associated tumors. Alterations in KMT2D, CREBBP, or ARID1A or in DNA damage response and repair genes were present at a significantly higher frequency in LS-UTUC. CIC, NOTCH1, NOTCH3, RB1, and CDKN1B alterations were almost exclusive to LS-UTUC. Although FGFR3 mutations were identified in both cohorts, the R248C hotspot mutation was highly enriched in LS-UTUC. CONCLUSION: LSand sporadic UTUCs have overlapping but distinct genetic signatures. LS-UTUC is associated with hypermutation and a significantly higher prevalence of FGFR3 R248C mutation. Prospective molecular characterization of patients to identify those with LS-UTUC may help guide treatment.
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    Tumor mutational signatures in sebaceous skin lesions from individuals with Lynch syndrome
    Georgeson, P ; Walsh, MD ; Clendenning, M ; Daneshvar, S ; Pope, BJ ; Mahmood, K ; Joo, JE ; Jayasekara, H ; Jenkins, MA ; Winship, IM ; Buchanan, DD (WILEY, 2019-07)
    BACKGROUND: Muir-Torre syndrome is defined by the development of sebaceous skin lesions in individuals who carry a germline mismatch repair (MMR) gene mutation. Loss of expression of MMR proteins is frequently observed in sebaceous skin lesions, but MMR-deficiency alone is not diagnostic for carrying a germline MMR gene mutation. METHODS: Whole exome sequencing was performed on three MMR-deficient sebaceous lesions from individuals with MSH2 gene mutations (Lynch syndrome) and three MMR-proficient sebaceous lesions from individuals without Lynch syndrome with the aim of characterizing the tumor mutational signatures, somatic mutation burden, and microsatellite instability status. Thirty predefined somatic mutational signatures were calculated for each lesion. RESULTS: Signature 1 was ubiquitous across the six lesions tested. Signatures 6 and 15, associated with defective DNA MMR, were significantly more prevalent in the MMR-deficient lesions from the MSH2 carriers compared with the MMR-proficient non-Lynch sebaceous lesions (mean ± SD=41.0 ± 8.2% vs. 2.3 ± 4.0%, p = 0.0018). Tumor mutation burden was, on average, significantly higher in the MMR-deficient lesions compared with the MMR-proficient lesions (23.3 ± 11.4 vs. 1.8 ± 0.8 mutations/Mb, p = 0.03). All four sebaceous lesions observed in sun exposed areas of the body demonstrated signature 7 related to ultraviolet light exposure. CONCLUSION: Tumor mutational signatures 6 and 15 and somatic mutation burden were effective in differentiating Lynch-related from non-Lynch sebaceous lesions.
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    Type 2 diabetes mellitus, blood cholesterol, triglyceride and colorectal cancer risk in Lynch syndrome
    Dashti, SG ; Li, WY ; Buchanan, DD ; Clendenning, M ; Rosty, C ; Winship, IM ; Macrae, FA ; Giles, GG ; Hardikar, S ; Hua, X ; Thibodeau, SN ; Figueiredo, JC ; Casey, G ; Haile, RW ; Gallinger, S ; Le Marchand, L ; Newcomb, PA ; Potter, JD ; Lindor, NM ; Hopper, JL ; Jenkins, MA ; Win, AK (NATURE PUBLISHING GROUP, 2019-11-12)
    BACKGROUND: Type 2 diabetes mellitus and high total cholesterol and triglycerides are known to be associated with increased colorectal cancer risk for the general population. These associations are unknown for people with a germline DNA mismatch repair gene mutation (Lynch syndrome), who are at high risk of colorectal cancer. METHODS: This study included 2023 (56.4% female) carriers with a mismatch repair gene mutation (737 in MLH1, 928 in MSH2, 230 in MSH6, 106 in PMS2, 22 in EPCAM) recruited by the Colon Cancer Family Registry between 1998 and 2012. Weighted Cox regression was used to estimate the hazard ratios (HR) and 95% confidence intervals (CI) for the associations between self-reported type 2 diabetes, high cholesterol, triglyceride and colorectal cancer risk. RESULTS: Overall, 802 carriers were diagnosed with colorectal cancer at a median age of 42 years. A higher risk of colorectal cancer was observed in those with self-reported type-2 diabetes (HR 1.92; 95% CI, 1.03-3.58) and high cholesterol (HR 1.76; CI 1.23-2.52) compared with those without these conditions. There was no evidence of high triglyceride being associated with colorectal cancer risk. CONCLUSION: For people with Lynch syndrome, self-reported type-2 diabetes mellitus and high cholesterol were associated with increased colorectal cancer risk.
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    Cancer Risks for PMS2-Associated Lynch Syndrome
    ten Broeke, SW ; van der Klift, HM ; Tops, CMJ ; Aretz, S ; Bernstein, I ; Buchanan, DD ; de la Chapelle, A ; Capella, G ; Clendenning, M ; Engel, C ; Gallinger, S ; Gomez Garcia, E ; Figueiredo, JC ; Haile, R ; Hampel, HL ; Hopper, JL ; Hoogerbrugge, N ; Doeberitz, MVK ; Le Marchand, L ; Letteboer, TGW ; Jenkins, MA ; Lindblom, A ; Lindor, NM ; Mensenkamp, AR ; Moller, P ; Newcomb, PA ; van Os, TAM ; Pearlman, R ; Pineda, M ; Rahner, N ; Redeker, EJW ; Olderode-Berends, MJW ; Rosty, C ; Schackert, HK ; Scott, R ; Senter, L ; Spruijt, L ; Steinke-Lange, V ; Suerink, M ; Thibodeau, S ; Vos, YJ ; Wagner, A ; Winship, I ; Hes, FJ ; Vasen, HFA ; Wijnen, JT ; Nielsen, M ; Win, AK (AMER SOC CLINICAL ONCOLOGY, 2018-10-10)
    PURPOSE: Lynch syndrome due to pathogenic variants in the DNA mismatch repair genes MLH1, MSH2, and MSH6 is predominantly associated with colorectal and endometrial cancer, although extracolonic cancers have been described within the Lynch tumor spectrum. However, the age-specific cumulative risk (penetrance) of these cancers is still poorly defined for PMS2-associated Lynch syndrome. Using a large data set from a worldwide collaboration, our aim was to determine accurate penetrance measures of cancers for carriers of heterozygous pathogenic PMS2 variants. METHODS: A modified segregation analysis was conducted that incorporated both genotyped and nongenotyped relatives, with conditioning for ascertainment to estimates corrected for bias. Hazard ratios (HRs) and corresponding 95% CIs were estimated for each cancer site for mutation carriers compared with the general population, followed by estimation of penetrance. RESULTS: In total, 284 families consisting of 4,878 first- and second-degree family members were included in the analysis. PMS2 mutation carriers were at increased risk for colorectal cancer (cumulative risk to age 80 years of 13% [95% CI, 7.9% to 22%] for males and 12% [95% CI, 6.7% to 21%] for females) and endometrial cancer (13% [95% CI, 7.0%-24%]), compared with the general population (6.6%, 4.7%, and 2.4%, respectively). There was no clear evidence of an increased risk of ovarian, gastric, hepatobiliary, bladder, renal, brain, breast, prostate, or small bowel cancer. CONCLUSION: Heterozygous PMS2 mutation carriers were at small increased risk for colorectal and endometrial cancer but not for any other Lynch syndrome-associated cancer. This finding justifies that PMS2-specific screening protocols could be restricted to colonoscopies. The role of risk-reducing hysterectomy and bilateral salpingo-oophorectomy for PMS2 mutation carriers needs further discussion.
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    Ability of known susceptibility SNPs to predict colorectal cancer risk for persons with and without a family history
    Jenkins, MA ; Win, AK ; Dowty, JG ; MacInnis, RJ ; Makalic, E ; Schmidt, DF ; Dite, GS ; Kapuscinski, M ; Clendenning, M ; Rosty, C ; Winship, IM ; Emery, JD ; Saya, S ; Macrae, FA ; Ahnen, DJ ; Duggan, D ; Figueiredo, JC ; Lindor, NM ; Haile, RW ; Potter, JD ; Cotterchio, M ; Gallinger, S ; Newcomb, PA ; Buchanan, DD ; Casey, G ; Hopper, JL (SPRINGER, 2019-10)
    Before SNP-based risk can be incorporated in colorectal cancer (CRC) screening, the ability of these SNPs to estimate CRC risk for persons with and without a family history of CRC, and the screening implications need to be determined. We estimated the association with CRC of a 45 SNP-based risk using 1181 cases and 999 controls, and its correlation with CRC risk predicted from detailed family history. We estimated the predicted change in the distribution across predefined risk categories, and implications for recommended screening commencement age, from adding SNP-based risk to family history. The inter-quintile risk ratio for colorectal cancer risk of the SNP-based risk was 3.28 (95% CI 2.54-4.22). SNP-based and family history-based risks were not correlated (r = 0.02). For persons with no first-degree relatives with CRC, screening could commence 4 years earlier for women (5 years for men) in the highest quintile of SNP-based risk. For persons with two first-degree relatives with CRC, screening could commence 16 years earlier for men and women in the highest quintile, and 7 years earlier for the lowest quintile. This 45 SNP panel in conjunction with family history, can identify people who could benefit from earlier screening. Risk reclassification by 45 SNPs could inform targeted screening for CRC prevention, particularly in clinical genetics settings when mutations in high-risk genes cannot be identified. Yet to be determined is cost-effectiveness, resources requirements, community, patient and clinician acceptance, and feasibility with potentially ethical, legal and insurance implications.
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    Cancer Risks for PMS2-Associated Lynch Syndrome (vol 29, pg 2961, 2018)
    ten Broeke, SW ; van der Klift, HM ; Tops, CMJ ; Aretz, S ; Bernstein, I ; Buchanan, DD ; de la Chapelle, A ; Capella, G ; Clendenning, M ; Engel, C ; Gallinger, S ; Garcia, EG ; Figueiredo, JC ; Haile, R ; Hampel, HL ; van Hest, L ; Hopper, JL ; Hoogerbrugge, N ; Doeberitz, MVK ; Le Marchand, L ; Letteboer, TGW ; Jenkins, MA ; Lindblom, A ; Lindor, NM ; Mensenkamp, AR ; Moller, P ; Newcomb, PA ; van Os, TAM ; Pearlman, R ; Pineda, M ; Rahner, N ; Redeker, EJW ; Olderode-Berends, MJW ; Rosty, C ; Schackert, HK ; Scott, R ; Senter, L ; Spruijt, L ; Steinke-Lange, V ; Suerink, M ; Thibodeau, S ; Vos, YJ ; Wagner, A ; Winship, I ; Hes, FJ ; Vasen, HFA ; Wijnen, JT ; Nielsen, M ; Win, AK (AMER SOC CLINICAL ONCOLOGY, 2019-03-20)
    This corrects the article "Cancer Risks for PMS2-Associated Lynch Syndrome" in volume 36 on page 2961.