Fluorescence-based Multiplex PCR-Single Strand Conformation Polymorphism (SSCP) Analysis of 16S Ribosomal DNA Using Capillary Electrophoresis

The rRNA genetic locus is found in all prokaryotic organisms, and is highly conservative, although its relatively stable variations are found frequently in different bacteria. The utility of this locus as a taxonomic and phylogenetic tool has been reported widely. This study, aimed at 16S rRNA gene (16S rDNA) and with the help of biomolecular methods, attempted to achieve the goal of rapid identification of common pathogens. In this study, 333 clinical isolated pathogenic bacteria were collected. Two pairs of primers were chosen and labeled with different fluorescent dyes and then used to amplify the genomic DNA extracted from bacteria. The PCR products were then detected by capillary electrophoresis-single strand conformation polymorphism (CE-SSCP). In order to pursue higher resolution and peak-separation effect, a high efficient separating medium, liner polyacrylamidedel (LPA), was put to use in this study. Finally, every bacteria colony generated distinct patterns from each other, which were easily to be used for identification. These results indicated that PCR-CE-SSCP was a rapid identification method for bacterial identification, with the aspects of high efficiency and high precision. Compared with traditional method, this technology is of great utility for clinical use especially for its high sensitivity.

Application of PCR-SSCP in detecting rpoB drug resistant gene polymorphism of M. tuberculosis L-form from pneumoconiosis patients with tuberculosis

Objective: To study the relationship between the polymorphism of drug resistant gene rpoB and drug resistance against rifampicin(RFP) of M. tuberculosis L-forms, and to evaluate its clinical application. Methods: A total of 52 clinical isolated strains of M. tuberculosis L-forms were collected. rpoB gene polymorphism was analyzed by polymerase chain reaction and single-strand conformation polymorphism (PCR-SSCP) and conventional antimicrobial susceptibility test (AST). Their results were compared. Results: AST results showed that 38 of 52 clinical isolated strains were drug resistance (73.08％),while PCR-SSCP indicated 65.38％ (32/52) rpoB gene polymorphism. There was no statistic significance(χ2= 2.4914) between the 2 methods. Conclusion:Combined the application of PCR-SSCP with AST in detecting rpoB drug resistant gene polymorphism of M. tuberculosis L-form from pneumoconiosis patients with tuberculosis may have advantages at earlier diagnosis and guidance of clinical medications.

Interleukin-10 promoter polymorphisms in patients with hepatitis B virus infection or hepatocellular carcinoma in Chinese Han ethnic population

BACKGROUND: Since single nucleotide polymorphisms (SNPs) can serve as gene markers, polymorphism profiles may help scientists to identify the full collection of genes that contribute to the development of complex diseases such as cancer. The distribution of interleukin-10 (IL-10) promoter polymorphisms in Chinese Han ethnic patients with hepatitis B virus (HBV) infection and hepatocellular carcinoma (HCC) was investigated in this study. METHODS: The polymorphisms of IL-10 promoter region were detected by pulymerase chain reaction-single strand conformation polymorphism (PCR-SSCP) and sequencing. Sixty-six health controls, 42 patients with HBV infection, 30 HCC patients, and cell line SMMC-7721 were examined this way. RESULTS: Polyrnorphisms of T/C or T/N on-872 site occurred frequently in Han ethnic population. Pulyrnorphisms were detected in HBV and HCC patients and cell line SMMC-7721. The hotspot among the pulymorphisms was inserting base A between-1058 and-1057. CONCLUSION: Polymorphisms of IL-10 promoter in HBV and HCC patients may be associated with HBV infection and HCC development.

Single nucleotide polymorphisms in the CDH17 gene of colorectal carcinoma

AIM:To investigate the relationship between c.343A>G and c.2216A>C polymorphism sites in the CDH17 gene and colorectal carcinoma.METHODS:Ninety-three non-consanguineous colorectal carcinoma patients admitted to the Department of Oncology at the First Affiliated Hospital of Zhengzhou University were included in this study.Ninety-three peripheral venous blood samples,of approximately one milliliter from each patient,were collected betweenDecember 2009 and August 2010.The genomic DNA of these peripheral venous blood samples were extracted and purified using a Fermentas Genomic DNA Purification Kit(Fermentas,CA) according to the manufacturer' s protocol.The single nucleotide polymorphisms(SNPs) of the liver-intestine cadherin(CDH17) gene c.343A>G and c.2216A>C were determined by the polymerase chain reaction-single strand conformation polymorphism method(PCR-SSCP) in 93 peripheral venous blood samples from patients suffering with colorectal carcinoma.Typical samples that showed different migration bands in SSCP were confirmed by sequencing.Directed DNA sequencing was used to check the correctness of the genotype results from the PCR-SSCP method.RESULTS:There was a significant association between the c.2216 A>C SNPs of the CDH17 gene and the tumor-node-metastasis(TNM) grade,as well as with lymph node status,in 93 peripheral venous blood samples from colorectal carcinoma patients.The genotype frequencies of A/C,A/A,and C/C were 12.90%,33.33% and 53.76%,respectively.There was a significant correlation between lymph node metastasis,TNM grade,and the genotype distribution(P < 0.05).The C/C genotype raised the risk of lymph node metastasis and the TNM grade.There was a significant difference in the TNM grade and lymph node metastasis between the A/A and C/C genotypes(P = 0.003 and P = 0.013,respectively).Patients with colorectal carcinoma carrying the C allele tended to have a higher risk of lymph node metastasis and have a higher TNM grade.The difference between the TNM grades,as well as the lymph node metastasis of the two alleles,was statistically significant(P < 0.01).CONCLUSION:The SNPs of the CDH17 gene c.2216 A>C might be clinically important in the prognosis of colorectal carcinoma.

PCR-SSCP及克隆测序法研究燃煤型砷中毒患者p53基因突变与皮肤癌的关系

[目的 ]分析燃煤型砷中毒患者外周血中p5 3基因突变情况。 [方法 ]采用聚合酶链反应 单链构象多态性(PCR -SSCP)技术对 60例燃煤型砷中毒患者外周血中p5 3基因 5～ 8外显子的突变情况进行初筛 ,并进一步克隆测序 ,以确定突变位点及类型。 [结果 ]癌变组p5 3基因突变率为 3 0 % ( 3 /10 ) ;癌前组为 16.67% ( 2 /12 ) ;一般病变组未发现突变 ( 0 /3 8)。对筛查出来的 5例突变阳性者进行克隆测序 ,突变均为G :C→A :T的转换 ,分别位于密码子 14 3、14 6及 15 1。[结论 ]燃煤型砷中毒患者外周血中p5 3基因突变的检出 。

常见食源性感染致病菌属、种用PCR-RFLP及PCR-SSCP技术鉴定探讨

【目的】探讨运用聚合酶链反应邛艮制性片段长度多态性分析(PCR-RFLP)和聚合酶链反应-单链构象多态性分析(PCR-SSCP)进行食源性感染常见致病菌属种鉴定的可行性。【方法】选择细菌23S rDNA基因作为鉴别细菌属的靶基因,通过设计合适的通用引物进行PCR扩增,并对13属食源性感染常见致病菌和5种不同血清型大肠杆菌扩增产物的酶切片段进行RFLP分析和SSCP分析。【结果】运用通用引物可以扩增出13 属食源性感染常见致病菌的23S rDNA基因HpaⅡ酶切产物的RFLP分析表明,不同种属的致病菌表现出不同的RFLP图谱,利于进行细菌属的鉴定。不同种属食源性感染常见致病菌SSCP图谱变异性更大,不利于进行种属间鉴别。对5种不同血清型大肠杆菌的23S rDNA基因扩增产物的RFLP和SSCP分析表明,不同血清型大肠杆菌表现出相似的RFLP图谱。SSCP图谱的变异性较大,这有利于进行血清型间鉴别甚至株间的鉴别。【结论】PCR-RFLP和PCR-SSCP具有应用于食源性感染常见致病菌种、属鉴别诊断的潜力。

应用RT/PCR-SSCP法分析传染性法氏囊病病毒的变异性

根据传染性法氏囊病病毒 ( IBDV) c DNA序列 ,在病毒 VP2区域设计 1对引物 ,应用 RT/PCR-SSCP方法对 4个不同时间及不同地域从传染性法氏囊病 ( IBD)病鸡法氏囊组织中分离的 IBDV分离物进行了分析 ,发现 4个 IBDV分离物的 SSCP图谱均存在明显差异。本试验表明 ,IBDV变异在我国普遍存在 ,SSCP方法可用于 IBDV的变异性分析。

PCR-SSCP技术在植物病毒学上的应用

聚合酶链式反应及单链构象多态性技术作为一种区分检测基因组之间微小差异的有效方法 ,具有快速、简便、灵敏和适用于大样品量筛选的特点 .本文详细介绍了该技术的条件优化及改进策略 .该技术在植物病毒学上主要应用于 :(1)分子变异 ;(2 )混合侵染的检测 ;(3)

绵羊PRNP等位基因PCR-SSCP分析条件的优化

为进行绵羊PRNP等位基因密码子136、154、171的多态性研究,建立适合于绵羊PRNP等位基因开放阅读框(ORF)内高变区PCR-SSCP分析方法,对凝胶浓度、交联度、甘油浓度、电泳电压、电泳时间、PCR产物与变性缓冲液比例、电泳缓冲液浓度、上样量等影响因素进行了优化试验。在优化中引入了正交试验法,以使优化过程简化,结果可靠。结果表明,交联度49∶1、甘油浓度0%、凝胶浓度12%、电泳电压200 V、PCR产物上样量≥2.0μL且<4.0μL、PCR产物与变性缓冲液比例1∶4、0.5×TBE缓冲液及4℃电泳45 h为最佳试验条件,据此建立了绵羊PRNP等位基因136、154、171密码子的PCR-SSCP分析方法。

PCR-SSCP检测非霍奇金淋巴瘤患者骨髓克隆性T细胞受体基因重排及其临床意义

背景与目的:进一步了解非霍奇金淋巴瘤(non-Hodgkinslymphoma,NHL)患者骨髓标本克隆T细胞受体(Tcellreceptor,TCR)基因重排情况及临床意义。方法:应用聚合酶链反应(polymerasechainreaction,PCR)联合单链构象多态性(single-strandconformationpolymorphism,SSCP)分析43例NHL患者骨髓标本TCRVγI-Jγ基因重排情况。结果:43例NHL患者有26例(60.5%)存在克隆性TCRVγI-Jγ基因重排。16例骨髓形态学检查未发现淋巴瘤细胞浸润者中有3例(18.8%)发现克隆性TCRVγI-Jγ基因重排,此3例患者分别于4～9个月后行骨髓形态检查时发现淋巴瘤细胞浸润;27例骨髓形态学检查有淋巴瘤细胞浸润者有23例(85.2%)存在克隆性TCRVγI-Jγ基因重排阳性。26例PCR扩增阳性病例经SSCP分析发现7例(26.9%)存在寡/亚克隆重排。7例存在寡/亚克隆重排患者经3～11个月有5例(71.4%)发展为白血病,存在寡/亚克隆重排NHL患者1年内转化为白血病的发生率显著高于无寡/亚克隆重排患者(10.5%)(P<0.005)。结论:应用PCR检测NHL患者骨髓标本克隆性TCRVγI-Jγ基因重排可较骨髓形态学检查更早发现NHL患者骨髓浸润微小病灶。具有寡/亚克隆NHL患者更易发展为白血病,还可发展为急性非淋巴细胞白血病。

PCR-SSCP法检测乙型肝炎病毒前C区基因变异

为探索一种快速、简便检测乙型肝炎病毒 (HBV)前 C区基因变异的方法 ,用聚合酶链反应 (PCR)技术扩增 94例乙肝患者血清 HBV前 C区基因片断 ,阳性扩增产物用单链构象多态性 (SSCP)法进行检测 ,对具有不同特征性电泳图谱的 PCR产物再以直接测序法加以核定 ,以辨别不同图谱与野生株、变异株或野生株、变异株混合感染之间的关系。结果显示 :有 86例患者 HBV前 C区 PCR扩增阳性 ,SSCP法检测发现有 3种常见的特征性电泳图谱 ,测序后证实 ,它们分别代表了野生株、变异株 (nt1896位 G→ A)及野生株、变异株混合感染的 SSCP图谱 ;在某些变异株图谱中 ,尚可见其它位点也存在变异 ,其中以 nt1899位 G→ A突变最为常见。提示 :以 PCR- SSCP技术检测 HBV前C区变异具有敏感性高 ,特异性强 ,简单、快捷、价廉等优点 ,而且特别适用于大样本的筛检 ,因此有应用价值 。

脊柱结核耐药性检测及耐药基因PCR-SSCP分析的应用价值

目的了解临床脊柱结核耐药情况,探讨耐药基因PCR-SSCP分析的临床应用价值。方法31例脊柱结核病灶应用BACTECMGIT960培养,所得临床分离株行药敏试验,对耐药基因rpsL、katG、rpoB行PCR-SS-CP分析。结果31例样本中27例培养阳性,其中18株存在不同程度耐药,总耐药率为66.67%。药物耐药率由高至低为链霉素10株(55.56%)、异烟肼8株(44.44%)、利福平7株(38.89%)、PZA3株(16.67%)。耐链霉素株rpsL突变率为70%,耐异烟肼株katG突变率为50%,耐利福平株rpoB突变率为71.43%。高浓度水平耐药株耐药基因突变率明显高于低浓度水平耐药株。结论常规药敏试验与耐药基因分析相结合可能更能准确地反应MTB的耐药情况。

应用PCR-SSCP检测转化细胞中p53基因突变

利用化学致突变物甲基丙烯酸环氧丙酯体外诱导人胚肺成纤维细胞，使之发生转化，分离转化细胞克隆。经ＰＣＲ特异性扩增ｐ５３基因外显子第５和第８，银染单链构象多态性（ＳＳＣＰ）分析，结果表明转化细胞中ｐ５３基因外显子第８发生突变，揭示出ｐ５３基因在化学致突变物诱导细胞转化中起着重要作用。

PCR-SSCP法检测结核分枝杆菌L型rpsL耐药基因

目的探索尘肺结核患者感染的结核分枝杆菌(MT)L型的耐药基因rpsL突变与耐受链霉素(SM)的关系。方法用PCR-SSCP方法检测rpsL基因,与采用常规SM药敏试验(AST法)的结果进行对比分析。结果采用AST法检测,52株结核分枝杆菌L型临床分离株中共有26株(50.0%)耐SM;PCR-SSCP法检出rpsL基因突变率为40.4%(21/52),2种方法检测耐药株的符合率为80.8%。结论结核杆菌L型对SM的耐药与rpsL基因突变有关。

PCR-SSCP检测大肠癌组织中p53、K-ras基因的突变

目的 探讨p5 3、K -ras基因突变与大肠癌发生、发展的关系。方法 应用PCR -SSCP方法检测 68例大肠癌和癌旁组织以及 2 0例正常组织中 p5 3、K -ras基因突变情况。 结果 大肠癌组织中 p5 3、K -ras基因突变率分别为 47.1% (3 2 68)和44 .1% (3 0 68) ,明显高于癌旁组织 (13 .2 % ,9 68;7.4% ,5 68) ,2 0例正常组织中未检出 p5 3、K -ras基因突变。伴有淋巴结及远处转移的大肠癌者 ,其 p5 3、K -ras基因突变率明显高于无淋巴结及远处转移者 ;p5 3、K -ras基因突变与大肠癌组织学类型无关。结论 p5 3、K -ras基因突变与大肠癌发生、发展有密切关系 ,其在细胞癌变中起重要作用 ,可作为评估大肠癌转移的分子生物学指标之一。

应用非同位素aPCR-SSCP法检测P53基因突变

建立一种非同位素的不对称聚合酶链反应－单链构象多态性技术（ａＰＣＲ－ＳＳＣＰ）：通过不对称ＰＣＲ（ａＰＣＲ）获得单链，普通ＰＡＧＥ电泳分离，经银染快速准确检出突变；应用这种方法，研究了４株鼻咽癌细胞株ＣＮＥ１，ＣＮＥ２，ＨＫ１和ＳＵＮＥ１中肿瘤抑制基因Ｐ５３基因突变，证实ＣＮＥ１，ＣＮＥ２在第８外显子，ＨＫ１在第５外显子有突变，并发现新建立的细胞株ＳＵＮＥ１存在第８外显子的突变。

PCR-SSCP快速检测脊柱结核耐药基因

目的了解临床脊柱结核耐药情况,探讨耐药基因PCR-SSCP对临床的应用价值。方法 43例脊柱结核患者结核肉芽组织应用BacT/ALERT 3D结核分支杆菌快速培养系统培养,所得临床分离株行药敏试验,对耐药基因katG、r p s L行PCR-SSCP。结果 43例结核肉芽组织标本培养后19例阳性,其中6株存在不同程度耐药,总耐药率为31%。耐异烟肼株katG突变率为10%,耐链霉素株rpsL突变率为21%,耐药基因检测平均用时为14h。结论 PCR-SSCP可快速检测脊柱结核耐药基因,与常规药敏试验结合可更能准确地反应脊柱结核患者的耐药情况。

肺癌患者hPARP-1基因突变PCR-SSCP检测

目的用聚合酶链反应-单链构象多态性(PCR-SSCP)技术研究肺癌患者聚腺苷二磷酸核糖聚合酶-1(hPARP-1)基因突变情况,寻找与肺癌发生相关的分子标记物。方法收集广东地区220名健康人群和106例肺癌病人的基础资料及血液标本,常规酚-氯法抽提血液DAN,用PCR单链构象多态性(SSCP)法检测hPARP-1基因第13,17和20外显子突变情况,并进行DNA序列分析。结果检测出5例肺癌病人在hPARP-1基因第17外显子有杂合性突变,为CAC→CGC的错义突变,即组氨酸→精氨酸。hPARP-1基因其余2个外显子未发现突变。结论PCR-SSCP是筛检基因突变的1种快速有效的方法,hPARP-1基因第17外显子上的突变可能是与肺癌发生相关的1种分子标记物。

PCR-SSCP技术在检测煤工尘肺并发肺结核患者感染的结核分枝杆菌耐药基因突变中的应用

目的探索尘肺结核患者感染的结核分枝杆菌(M.tuberculosis)耐药基因突变与耐药性的关系,及聚合酶链反应-单链构象多态性分析(PCR-SSCP)的临床应用价值。方法在102例淮南矿区煤工尘肺并发结核患者中分离出M.tuberculosis菌株32株,采用PCR-SSCP法检测katG、rpoB和rpsL基因突变,与采用常规药敏试验(AST)法检测的耐药结果进行对比分析。结果采用PCR-SSCP法检测katG、rpoB和rpsL基因,突变率分别为43.75%(14/32),53.13%(17/32)和31.25%(10/32);采用AST法检测INH、RFP和SM,耐药率分别为53.13%(17/32),65.63%(21/32)和40.63%(13/32),其中多耐药株19例(59.38%),包括耐3种药物的11例(42.31%),耐2种药的8例(30.77%),单耐药株7例(26.92%),敏感株6例,耐药率81.25%。PCR-SSCP法检出3个基因联合突变的有7株(7/26,26.92%),与AST法的符合率为63.64%(7/11);2个基因突变的6株(6/26,23.08%),符合率为50.00%(4/8);单基因突变的8株(8/26,30.77%),符合率为57.14%(4/7)。结论PCR-SSCP技术适用于淮南矿区煤工尘肺并发结核患者感染的M.tuberculosis katG、rpoB和rpsL耐药基因突变的筛选,将其与AST法联合应用,在指导临床用药方面具有着重要的意义。

PCR-SSCP法分析汉坦病毒在乳鼠中的基因变异

目的：研究汉坦病毒在感染乳鼠体内有无基因变异．方法：用陈株病毒感染Ｖｅｒｏ－Ｅ６细胞并继之感染３ｄ龄乳鼠，提取病毒ＲＮＡ并反转录成ｃＤＮＡ，以ＰＣＲ分别从感染细胞和乳鼠中克隆出病毒的部分Ｇ２编码区序列，继而用非变性聚丙烯酰胺凝胶电泳对之进行单链构象多态性（ＳＳＣＰ）分析．结果：从感染细胞和乳鼠中克隆出的此位置和大小完全相同的ｃＤＮＡ片段单链电泳构像明显不同，从感染乳鼠中克隆的基因片段单链电泳速率明显快于从感染细胞中克隆的相应基因片段．结论：汉坦病毒的基因序列可因寄生宿主的不同而发生变异．