Fecal microbial biomarkers combined with multi-target stool DNA test improve diagnostic accuracy for colorectal cancer

BACKGROUND Colorectal cancer(CRC)is a major global health burden.The current diagnostic tests have shortcomings of being invasive and low accuracy.AIM To explore the combination of intestinal microbiome composition and multi-target stool DNA(MT-sDNA)test in the diagnosis of CRC.METHODS We assessed the performance of the MT-sDNA test based on a hospital clinical trial.The intestinal microbiota was tested using 16S rRNA gene sequencing.This case-control study enrolled 54 CRC patients and 51 healthy controls.We identified biomarkers of bacterial structure,analyzed the relationship between different tumor markers and the relative abundance of related flora components,and distinguished CRC patients from healthy subjects by the linear discriminant analysis effect size,redundancy analysis,and random forest analysis.RESULTS MT-sDNA was associated with Bacteroides.MT-sDNA and carcinoembryonic antigen(CEA)were positively correlated with the existence of Parabacteroides,and alpha-fetoprotein(AFP)was positively associated with Faecalibacterium and Megamonas.In the random forest model,the existence of Streptococcus,Escherichia,Chitinophaga,Parasutterella,Lachnospira,and Romboutsia can distinguish CRC from health controls.The diagnostic accuracy of MT-sDNA combined with the six genera and CEA in the diagnosis of CRC was 97.1%,with a sensitivity and specificity of 98.1%and 92.3%,respectively.CONCLUSION There is a positive correlation of MT-sDNA,CEA,and AFP with intestinal microbiome.Eight biomarkers including six genera of gut microbiota,MT-sDNA,and CEA showed a prominent sensitivity and specificity for CRC prediction,which could be used as a non-invasive method for improving the diagnostic accuracy for this malignancy.

Multitarget stool DNA for colorectal cancer screening:A review and commentary on the United States Preventive Services Draft Guidelines

Multitarget stool DNA(mt-sDNA) testing was approved for average risk colorectal cancer(CRC) screening by the United States Food and Drug Administration and thereafter reimbursed for use by the Medicare program(2014).The United States Preventive Services Task Force(USPSTF) October 2015 draft recommendation for CRC screening included mt-s DNA as an "alternative" screening test that "may be useful in select clinical circumstances",despite its very high sensitivity for early stage CRC.The evidence supporting mt-s DNA for routine screening use is robust.The clinical efficacy of mt-s DNA as measured by sensitivity,specificity,life-years gained(LYG),and CRC deaths averted is similar to or exceeds that of the other more specifically recommended screening options included in the draft document,especially those requiring annual testing adherence.In a population with primarily irregular screening participation,tests with the highest point sensitivity and reasonable specificity are more likely to favorably impact CRC related morbidity and mortality than those depending on annual adherence.This paper reviews the evidence supporting mt-s DNA for routine screening and demonstrates,using USPSTF's modeling data,that mt-s DNA at three-year intervals provides significant clinical net benefits and fewer complications per LYG than annual fecal immunochemical testing,high sensitivity guaiac based fecal occult blood testing and 10-year colonoscopy screening.

Multitarget stool DNA tests increases colorectal cancer screening among previously noncompliant Medicare patients

AIM To determine the uptake of noninvasive multitarget stool DNA (mt-s DNA) in a cohort of colorectal cancer(CRC) screening non-compliant average-risk Medicare patients.METHODS This cross sectional primary care office-based study examined mt-s DNA uptake in routine clinical practice among 393 colorectal cancer screening non-compliant Medicare patients ages 50-85 ordered by 77 physicians in a multispecialty group practice (USMD Physician Services, Dallas, TX) from October, 2014-September, 2015. Investigators performed a Health Insurance Portability and Accountability Act compliant retrospective review of electronic health records to identify mt-s DNA use in patients who were either > 10 years since last colonoscopy and/or > 1 year since last fecal occult blood test. Test positive patients were advised to get diagnostic colonoscopy and thereafter patients were characterized by the most clinically significant lesion documented on histopathology of biopsies or excisional tissue. Descriptive statistics were employed. Key outcome measures included mt-s DNA compliance and diagnostic colonoscopy compliance on positive cases.RESULTS Over 12 mo, 77 providers ordered 393 mt-sD NA studies with 347 completed (88.3% compliance). Patient mean age was 69.8 (50-85) and patients were 64% female. Mt-sD NA was negative in 85.3%(296/347) and positive in 14.7%(51/347). Follow-up colonoscopy was performed in 49 positive patients (96.1% colonoscopy compliance) with two patients lost to follow up. Index findings included: colon cancer(4/49, 8.2%), advanced adenomas (21/49, 42.9%), non-advanced adenomas(15/49, 30.6%), and negative results (9/49, 18.4%). The positive predictive value for advanced colorectal lesions was 51.0% and for any colorectal neoplasia was 81.6%. The mean age of patients with colorectal cancer was 70.3 and all CRC's were localized Stage Ⅰ(2) and Stage Ⅱ (2), three were located in the proximal colon and one was located in the distal colon.CONCLUSION Mt-s DNA provided medical benefit to screening noncompliant Medicare population. High compliance with mt-s DNA and subsequent follow-up diagnostic colonoscopy identified patients with clinically critical advanced colorectal neoplasia.

Patient perceptions of stool DNA testing for pan-digestive cancer screening:A survey questionnaire

AIM: To explore patient interest in a potential multi-organ stool-DNA test (MUST) for pan-digestive cancer screening.

Stool-based DNA testing,a new noninvasive method for colorectal cancer screening,the first report from Iran

AIM： To detect tumor-associated DNA changes in stool samples among Iranian patients with colorectal cancer （CRC） compared to healthy individuals using BAT-26, p16 hypermethylation and long DNA markers. METHODS： Stool DNA was isolated from 45 subjects including 25 CRC patients and 20 healthy individuals using a new, fast and easy extraction method. Long DNA associated with tumor was detected using polymerase chain reaction method. Microsatellite studies were performed utilizing denaturating polyacrylamide gel to determine the instability of BAT-26. Methylation status of p16 promoter was analyzed using methylation-specific PCR （MSP）. RESULTS： The results showed a significant difference in existence of long DNA （16 in patients vs 1 in controls, P 〈 0.001） and p16 （5 in patients vs none in controls, P = 0.043） in the stool samples of two groups. Long DNA was detected in 64% of CRC patients; whereas just one of the healthy individuals was positive for Long DNA. p16 methylation was found in 20% of patients and in none of healthy individuals. Instability of BATo26 was not detected in any of stool samples. CONCLUSION： We could detect colorectal cancer related genetic alterations by analyzing stool DNA with a sensitivity of 64% and 20% and a specificity of 95% and 100% for Long DNA and p16 respectively. A non- invasive molecular stool-based DNA testing can provide a screening strategy in high-risk individuals. However, additional testing on more samples is necessary from Iranian subjects to determine the exact specificity and sensitivity of these markers.

Stool DNA-based versus colonoscopy-based colorectal cancer screening: Patient perceptions and preferences

Objective:Stool DNA(sDNA)tests offer a noninvasive form of colon cancer screening for pa-tients,and although the test is expected to increase uptake of colon cancer screening,it is unknown if patients’perceptions of the sDNA test differ according to race and other patient characteristics.Methods:We conducted a self-administered survey of patients undergoing both a colonoscopy and an sDNA test to evaluate perceptions of sDNA testing.Results:Of the 613 participants who were sent surveys,423 responded(69%response rate).Respondents self-identified as African American(n=127,30%),Caucasian(n=284,67%),and other ethnicity(n=12,3%).In general,participants found the sDNA test more suitable than a colonos-copy(n=309,75%).In univariate analyses,a higher percentage of Caucasians as compared with African Americans found the sDNA test more suitable than a colonoscopy(89%vs.76%,p<0.01),and more Caucasians than African Americans preferred the sDNA test(43%vs.32%,p<0.05).Ad-justment for covariates reduced these racial differences to no significance.A family history of colo-rectal cancer remains a significant factor for patient’s preferences for screening regardless of race.Conclusions:Our study shows no racial differences in the perception of and preference for sDNA testing for colon screening.Intervention to increase the uptake of sDNA testing may help reduce racial disparities in colorectal cancer.

粪便DNA甲基化检测在结直肠癌早期诊断中的研究进展

粪便基因甲基化作为一种新的、敏感度较高、特异性中等的无创性结直肠肿瘤标志物,能根据其阳性结果对疑似病例进行进一步检测,可作为筛查诊断结直肠肿瘤的一种重要的辅助手段。目前已有较多研究报道检测粪便中基因异常甲基化对于早期结直肠癌(colorectal cancer,CRC)筛查有较高的敏感性和特异性,但尚无任何一种甲基化基因真正地应用于临床实践。本文对目前结直肠癌早期粪便DNA甲基化检测的国内外相关研究成果进行综述,总结粪便甲基化检测的潜在临床价值。

DNA甲基化在肿瘤无创性分子诊断中的研究进展

DNA甲基化是真核细胞基因组最常见的一种表观遗传学修饰。DNA甲基化异常在肿瘤的发生、发展过程中扮演重要角色。研究显示DNA甲基化是一类潜力很大的肿瘤标志物。肿瘤特异性的DNA甲基化标志物可从肿瘤患者血清/血浆、尿液、粪便和支气管肺泡灌洗液中检出,为进行肿瘤无创性诊断DNA甲基化检测提供了新思路。本文对DNA甲基化在恶性肿瘤早期诊断的研究进展作一综述。

粪便DNA检测筛查大肠癌的进展

大肠癌的发生发展是一个多基因作用的多阶段过程,主要涉及的基因包括APC、K-Ras、p53、DCC、BAT26等。粪便DNA检测筛查大肠癌是20世纪90年代出现的一种新方法,具有非侵入性、患者依从性好、敏感性和特异性高等优点。经过十几年的发展,粪便DNA检测已由早期的单基因检测发展到多基因联合检测,检出率也有较大的提高。随着分子生物学技术的日臻完善,粪便DNA检测显现出巨大潜力,为大肠癌的筛查开拓了更广阔的空间。

Gene mutations in stool from gastric and colorectal neoplasia patients by next-generation sequencing

AIM To study cancer hotspot mutations by next-generation sequencing(NGS) in stool DNA from patients with different gastrointestinal tract(GIT) neoplasms. METHODS Stool samples were collected from 87 Finnish patients diagnosed with various gastric and colorectal neoplasms, including benign tumors, and from 14 healthy controls. DNA was isolated from stools by usingthe PSP~? Spin Stool DNA Plus Kit. For each sample, 20 ng of DNA was used to construct sequencing libraries using the Ion AmpliS eq Cancer Hotspot Panel v2 or Ion AmpliS eq Colon and Lung Cancer panel v2. Sequencing was performed on Ion PGM. Torrent Suite Software v.5.2.2 was used for variant calling and data analysis.RESULTS NGS was successful in assaying 72 GIT samples and 13 healthy controls, with success rates of the assay being78% for stomach neoplasia and 87% for colorectal tumors. In stool specimens from patients with gastric neoplasia, five hotspot mutations were found in APC,CDKN2 A and EGFR genes, in addition to seven novel mutations. From colorectal patients, 20 mutations were detected in AKT1, APC, ERBB2, FBXW7, KIT, KRAS,NRAS, SMARCB1, SMO, STK11 and TP53. Healthy controls did not exhibit any hotspot mutations, except for two novel ones. APC and TP53 were the most frequently mutated genes in colorectal neoplasms, with five mutations, followed by KRAS with two mutations.APC was the most commonly mutated gene in stools of patients with premalignant/benign GIT lesions.CONCLUSION Our results show that in addition to colorectal neoplasms,mutations can also be assayed from stool specimens of patients with gastric neoplasms.

粪便中日本血吸虫虫卵DNA的提取及PCR检测方法的优化

目的建立一套系统、完整的粪便日本血吸虫虫卵DNA提取法及PCR优化体系。方法利用蛋白酶K和苯酚法从感染日本血吸虫尾蚴的家兔粪便中提取DNA,根据日本血吸虫基因(AF00369)设计特异性引物,以粪便中提取的DNA为模板,采用PCR方法扩增目的基因片段,对PCR方法的各种反应条件进行优化并采用有限稀释法推测PCR检测法可检测到的最低虫卵数。结果以感染家兔的粪便中提取的DNA为模板,用PCR方法可扩增到分子量大小约为400 bp的特异性条带,测序结果经BLAST工具进行分析,与日本血吸虫基因(AF00369)比对的同源性为96%;25μl PCR反应体系的最优化反应条件:MgCl2 1.5μl;dNTP 0.5μl;引物1.0μl;DNA模板5.0μl;Taq DNA聚合酶0.5μl。扩增程序为:94℃预变性5min、94℃变性30s、53℃退火30s、72℃延伸30s,30个循环、72℃延伸7min、4℃保存。PCR检测法可检测到的最低虫卵数为0.015个。结论成功建立感染家兔粪便中虫卵DNA的提取方法及PCR血吸虫基因片段检测方法,同时对PCR反应条件进行优化,为从分子角度检测日本血吸虫虫卵DNA提供科学的实验依据。

肺结核患者粪便TB-DNA提取方法的应用比较

目的比较煮沸裂解法、酚/氯仿法和试剂盒法3种DNA提取法在肺结核患者粪便标本中检测TB-DNA的应用效果。方法收集肺结核患者粪便标本,分别用煮沸裂解法、酚/氯仿法和试剂盒法提取DNA,比较其TB-DNA实时荧光聚合酶链反应(PCR)扩增的检测阳性率及扩增效率,分析不同方法的差异。结果对于痰抗酸涂片阴性患者的粪便标本,3种方法均未测到有TB-DNA扩增。痰抗酸涂片阳性患者的粪便标本,煮沸裂解法、酚/氯仿法和试剂盒法的TB-DNA检出率分别为45%、70%和80%。酚/氯仿法与试剂盒法TB-DNA的定量结果比较,存在显著性差异,试剂盒法提取扩增效果显著强于酚/氯仿法。结论试剂盒法可有效去除粪便标本中的PCR抑制物,TB-DNA检出率和定量结果明显优于煮沸裂解法和酚/氯仿法,对于无法产生痰或咳出痰的肺结核患者的实验室诊断具有较高的应用价值。

广州试点开展多靶点粪便FIT-DNA联合检测用于大肠癌筛查的结果分析

目的对2017年广州市在白云、越秀、海珠3区试点开展大肠癌初筛阳性人群进行多靶点粪便FIT-DNA联合检测(常卫清)筛查结果进行分析和总结,为广州市大肠癌筛查工作的进一步推进提供参考数据。方法对2015-2017年大肠癌初筛阳性[问卷评估阳性或者免疫法便隐血检测(胶体金法)大便隐血(FIT)阳性]多次动员仍未接受肠镜检查的高危人群,动员接受新型筛查技术-多靶点粪便FIT-DNA联合检测(常卫清),检测阳性者进一步建议进行肠镜检查;然后,统计分析不同地区、性别、年龄组的多靶点粪便FIT-DNA联合检测阳性率、肠镜检查依从性以及肠镜检查异常情况。结果870例初筛阳性入组,男332例,女538例。841例进行多靶点粪便FIT-DNA联合检测(常卫清),阳性率为13.91%(117/841),其中白云、越秀、海珠3个区阳性率分别为13.87%(33/238)、14.35%(31/216)、13.66%(53/387),男性和女性的阳性率分别为19.00%(61/321)和10.77%(56/520),不同年龄组<40、40~49、50~59、60~69、70~74、>74岁的阳性率分别为0.00%(0/3)、6.25%(2/32)、11.21%(25/223)、15.21%(66/434)、16.52%(19/115)、22.73%(5/22)。55例完成肠镜检查,肠镜依从率为47.01%(55/117),其中白云、越秀、海珠3个区的肠镜依从率分别为33.33%(11/33)、87.10%(27/31)、32.08%(17/53),男性和女性的肠镜依从率为45.90%(28/61)和48.21%(27/56),不同年龄组50~59、60~69、70~74岁的肠镜依从率分别为44.00%(11/25)、51.52%(34/66)、21.05%(4/19)。45例随访到肠镜结果,30例检查结果异常,病变总检出率为66.67%(30/45),其中结直肠癌3例,腺瘤11例,息肉15例,肠炎1例。结论在大肠癌的筛查策略中,建议对初筛阳性的高危人群引入多靶点粪便FIT-DNA联合检测(常卫清)进一步精筛,以提高进一步进行肠镜检查的依从性。

粪便DNA中MGMT、XAF1基因启动子甲基化联合检测在结直肠癌筛查中的应用研究

目的使用甲基化特异性PCR(MSP)方法检测粪便DNA中O6-甲基鸟嘌呤-DNA甲基转移酶(MGMT)、X染色体连锁凋亡抑制蛋白相关因子1(XAF1)基因启动子甲基化情况,并探讨其在结直肠肿瘤诊断中的意义。方法收集40例结直肠腺癌、40例腺瘤性息肉、52例正常对照住院患者粪便标本,使用试剂盒提取其粪便中肠道脱离细胞DNA,通过MSP方法检测其MGMT、XAF1基因启动子甲基化情况。结果 MGMT、XAF1基因启动子甲基化在结直肠腺癌中的阳性率分别为50.0%、55.9%;在腺瘤性息肉中的阳性率分别为42.1%、52.6%;二者联合检测在结直肠腺癌及腺瘤性息肉中的阳性率分别为73.5%、68.4%;特异性为52.0%。结直肠腺癌患者粪便中粪便潜血阳性率为35.3%,CEA阳性率为35.3%。结论通过试剂盒提取粪便DNA具有较高成功率;粪便DNA中MGMT、XAF1基因启动子甲基化状态用于检测结直肠腺癌及腺瘤性息肉具有较高的敏感性。检测粪便基因甲基化有望成为CRC高风险人群筛查的一个重要途径。

介绍一种改量的粪便细菌基因组DNA提取试验方法

目的观察改变细菌裂解温度对提取粪便细菌基因组DNA量和纯度的影响。方法收集10例肝硬化患者粪便,每例患者粪便等分成两份,再随机分成两组。采用QIAamp DNA Stool Mini Kit试剂盒(国际通用粪便细菌基因组DNA提取试剂盒)进行抽提,一组(A组)按照试剂盒说明书温度要求进行粪便细菌基因组DNA提取,一组(B组)对试剂盒细菌裂解温度改良后再进行提取。结果与按照试剂盒说明书温度进行提取组相比,改变细菌裂解温度后粪便基因组DNA提取量明显增高(P<0.05),而粪便基因组DNA提取纯度(OD260/280、OD260/230)无明显变化(P>0.05)。结论改变细菌裂解温度能明显提高粪便细菌基因组DNA提取量,而不改变粪便细菌基因组DNA的提取纯度。该方法可以解决因粪便采样量少导致粪便基因组DNA提取量不足的问题。

粪便DNA中联合SFRP1及SEPT9基因甲基化检测对老年性结直肠癌早期诊断的临床研究

目的探讨粪便DNA中联合分泌型卷曲相关蛋白1(SFRP1)及胞裂蛋白9(SEPT9)基因甲基化检测对老年性结直肠癌(CRC)早期诊断的临床价值。方法选取我院从2016年1月至2016年9月确诊的35例年龄>60岁CRC患者为研究组,选取同期35例>60岁正常体检者为对照组。提取CRC患者和正常体检者粪便DNA,采用甲基化特异性PCR(MSP)技术分别检测SFRP1及SEPT9基因的甲基化状态;比较CRC患者单基因和联合双基因甲基化检出率的差异,以及CRC患者联合双基因甲基化检出率与对照组的差异;分析CRC患者SFRP1或SEPT9基因甲基化与临床病理特征(如年龄、性别、肿瘤位置)的关系。结果 CRC患者粪便DNA中SFRP1及SEPT9基因甲基化检出率分别为45.71%(16/35)和51.43%(18/35),均显著高于对照组的8.57%(3/35)和14.29%(5/35),差异均有统计学意义(P<0.01);联合双基因检测结果显示,82.86%(29/35)的CRC患者粪便DNA中至少存在一个基因的甲基化,显著高于单基因检出率(P<0.01),亦高于对照组的17.14%(6/35),差异有统计学意义(P<0.01)。CRC患者SFRP1或SEPT9基因甲基化与年龄、性别、肿瘤位置均无关(P>0.05)。结论粪便DNA中联合SFRP1及SEPT9基因甲基化检测比单基因检测更加敏感,对老年性CRC早期诊断具有重要的应用价值。

DNA methylation assay for colorectal carcinoma

Colorectal carcinoma(CRC) is a common cause of morbidity and mortality worldwide. Two pathogenic pathways are involved in the development of adenoma to CRC. The first pathway involves APC/β-catenin characterized by chromosomal instability resulting in the accumulation of mutations. The second pathway is characterized by lesions in DNA mismatch repair genes.Aberrant DNA methylation in selected gene promoters has emerged as a new epigenetic pathway in CRC development. CRC screening is the most efficient strategy to reduce death. Specific DNA methylation events occur in multistep carcinogenesis.Epigenetic gene silencing is a causative factor of CRC development. DNA methylations have been extensively examined in stool from CRC and precursor lesions. Many methylated genes have been described in CRC and adenoma, although no definite DNA methylation biomarkers panel has been established. Multiple DNA methylation biomarkers, including secreted frizzled-related protein 2, secreted frizzled-related protein 1, tissue factor pathway inhibitor 2, vimentin, and methylguanine DNA methyltransferase, have been further investigated, and observations have revealed that DNA methylation biomarkers exhibit with high sensitivity and specificity. These markers may also be used to diagnose CRC and adenoma in early stages. Real time polymerase chain reaction(q PCR) is sensitive, scalable, specific, reliable, time saving, and cost effective. Stool exfoliated markers provide advantages, including sensitivity and specificity. A stool q PCR methylation test may also be an enhanced tool for CRC and adenoma screening.

粪便样本中高纯度人源DNA富集提取方法

粪便肠脱落细胞DNA的提取是影响基因检测技术在结直肠癌筛查领域应用的关键。目的:通过对提取过程、试剂进行研究,开发高纯度人源DNA富集提取方法。方法:对粪便样本提取前均质化方式进行优化,并使用PVP高分子交联剂预处理均质化粪便上清。结果:颠倒混匀均质化方式可以显著降低微生物DNA的比例,实现人源DNA的相对富集;PVP高分子交联剂可以有效去除多糖、蛋白、胆盐等杂质,减少粪便DNA的PCR抑制;结直肠癌患者粪便DNA与癌组织样本DNA的重亚硫酸盐转化测序(BSP)结果中的甲基化特征一致。结论:优化后的粪便DNA富集提取产物PCR检测结果准确性良好,该提取方法可行性高。

多靶点粪便DNA、肠道菌群、癌胚抗原及水果摄入对结直肠癌风险的交互作用研究

目的探讨多靶点粪便DNA(MT-sDNA)、肠道菌群及饮食等环境因素之间的交互作用以及对结直肠癌的影响,为结直肠癌发病机制研究提供依据。方法选择宁波大学附属第一医院结直肠癌病例54例纳入病例组,同期健康体检者51人纳入对照组,通过问卷调查收集人口学信息、饮食和结直肠癌家族史等资料;检测MT-sDNA、肠道菌群,以及癌抗原19-9、癌胚抗原(CEA)等肿瘤标志物;采用多因子降维法、叉生分析法和相加交互作用模型分析MT-sDNA、肠道菌群、环境因素的交互作用对结直肠癌患病的影响。结果病例组年龄为(64.89±9.72)岁,男性20例,占37.04%,女性34例,占62.96%;对照组年龄为(53.94±10.33)岁,男性24人,占47.06%,女性27人,占52.94%。多因子降维法分析结果显示,同时有肠道菌群指数绝对值偏高和MT-sDNA阳性的人群患结直肠癌的风险较高(OR=3.782,95%CI:1.190~5.034)。叉生分析结果显示,MT-sDNA阳性与CEA>5μg/L的人群患结直肠癌的风险较高(OR=2.121,95%CI:1.162~4.033)。相加模型分析结果显示,MT-sDNA与CEA存在正相加交互作用(SI=3.687,95%CI:1.229~7.238),MT-sDNA与吃水果存在负相加交互作用(SI=0.145,95%CI:0.020~0.753)。结论MT-sDNA阳性可与肠道菌群指数偏高或CEA联合增加结直肠癌风险,吃水果可减少MT-sDNA阳性人群的结直肠癌风险。

联合检测vimentin和SFRP2甲基化在大肠癌筛查中的应用评价

目的评价在粪便样本中联合检测vimentin和SFRP2甲基化来筛查大肠癌的性能。方法搜集合格的新鲜粪便标本95例,其中40例大肠癌患者、25例进展期腺瘤患者和30例结肠镜阴性的正常人,应用甲基化特异性PCR(MSP)法检测vimentin和SFRP2甲基化状态,并与单个基因甲基化检测和粪隐血试验(FOBT)的诊断性能相比较是否有统计学差异。结果大肠癌组中vimentin和SFRP2甲基化阳性检出率分别为55.0%(22/40)和70.0%(28/40);进展期腺瘤组中为48.0%(12/25)和64.0%(16/25);正常对照组中为6.7%(2/30)和0(0/30)。在病例组中两基因联合检测的敏感性为83.1%(54/65),明显高于vimentin的52.3%(34/65)和SFRP2的67.7%(44/65),更要高于FOBT的27.7%(18/65)(均P<0.05)。而在正常对照组中两基因联合检测的特异性为93.3%(28/30),与vimentin的93.3%(28/30)和SFRP2的100%(30/30)以及FOBT的96.7%(29/30)相比均无明显差异(均P>0.05)。结论在大肠癌筛查中,联合检测粪便中vimentin和SFRP2基因甲基化状态明显优于单个基因和粪便潜血试验,具有潜在的应用价值。