Detection of Ratoon Stunting Disease in Virus-free Seedcane via Real-time Fluorescence Quantitative PCR

This study was to develop the real-time fluorescence quantitative PCR technique for detecting the ratoon stunting disease （RSD） in virus-free seedcane seedlings. Healthy tissue culture seedlings were obtained from six plants of sugarcane ROC22, which had been confirmed RSD-positive by detecting the sugarcane juice, by employing the sugarcane seedlings production protocol. Real-time fluorescence quantitative PCR was used to detect RSD pathogens in tissue culture sam- pies. The results showed that target fragment of RSD pathogens was not found in all 10 samples in real-time fluorescence quantitative PCR, with the Ct values of 37 - 39. The healthy tissue culture sugarcane seedlings do not carry RSD pathogens, indicating that adopting healthy seedcane seedlings production technique could thoroughly get rid of RSD pathogens.

Real-time fluorescent quantitative PCR非特异性扩增的研究进展

Real-time fluorescent quantitative PCR(RT-qPCR)因其高效快速、操作简便、高度敏感等优点获得广泛应用,但因其强大的放大功能而容易出现非特异性扩增的问题,尤其是荧光染料法中更加明显。文章对RT-qPCR的原理、非特异性扩增的发生因素、解决方案及该技术的应用前景进行了综述。

Development and Preliminary Application of SYBR Green I Real-Time Fluorescence Quantitative PCR Method for Detecting Porcine Parvovirus Virus

According to VP2 gene sequence of the porcine parvovirus virus strain NADL-2 （NC001718） available in GenBank （NC_001718）, a pair of specific primer was designed, and the target fragment of 431 bp was obtained by PCR amplification. The products were ligated with pMD18- T vector and then transformed into bacteria DH5α for recombinant plasmid extraction. After PCR identification and sequencing, recombinant plasmid was used as a standard template to establish the standard curve of SYBR Green I fluorescence quantitative PCR. Sensitivity test, specificity test and repeatability test were also determined. The results indicated that there was a good linear relationship between threshold cycle of the standard curve and template concentration, R2 =0.997 6. Tm ranged from 82.3 to 82.9 ℃, while the sensitivity was 72.1 copies/μl with good specificity and repeatability. The developed SYBR Green I real-time quantitative PCR method to detect PPV VP2 gene laid the basis for further studies on patho- oenesis, early clinical diaonosis of this virus and quantitative analysis of PPV infection.

Detection of Lactobacillus acidophilus in Fermented Material by Real-time Fluorescent Quantitative PCR

The species distinctive PCR primer of Lactobacillus acidophilus （ L. acidophilus） was designed according to 16S rRNA gene sequences of conunon Lac- tobacillus species in fermented material. Bacterial genome DNA of separated L. acidophilus in fermented sample was taken as template, and L. acidophilus in fer- mented material was conducted the quantitative determination by real-time quantitative PCR （RT-PCR）. Analysis on RT-PCR results shown that contents of L. aci- dophilus in the test sample reached 1.5 billion CFU / g. Test results shown that contents of L. acidophilus in fermented material could be detected accurately by the established RT-PCR method in the test. indicating that the established RT-PCR method could be aookued to the detection of L. acidophilus in fermented material.

Application of Real-time Fluorescent Quantitative PCR in Studies on Plants

Real-Lime fluorescent quantitative PCR is a method for quantitative analysis of gene expression developed in recent years, which has been widely used in various fields such as basic scientific research, clinical diagnosis, disease study, drug research and development since its appearance. It starts relatively late in study on plants, but has already been used for analysis of gene expression in plants and gene identification of exogenous genes. The principles or advantages and dis- advantages of real-time fluorescent quantitative PCR, or its potential problems and condition optimizations in tests were introduced in this study, and then the appli- cation and prospect of real-time fluorescent quantitative PCR in study on plants were also been discussed.

Establishment of a Real-time Fluorescent Quantitative PCR Assay for Detection of Genetically Modified Maize Line MON88017

In order to improve the standardized technical systems of quantitative analyses for genetically modified organisms （GMOs） and products, ensure bio-safety and reduce ecological risk in China, a real-time fluorescent quantitative PCR assay was established for detection of genetically modified maize line MON88017. The established method was evaluated based on the specificity, sensitivity, accuracy and measurement uncertainty. The results showed that the established method had strong specificity in detection of genetically modified maize line MON88017. 1.50% MON88017 sample was detected with 29 replica- tions. The average measured value （ 1. 541% ） was close to the actual value （ 1.50% ） and the relative deviation was 2.70%. The variation coefficient of the measured value was 0.110 g ; the recovery was 100.00% and the measurement uncertainty was 0. 096. The limit of detection for genetically modified maize line MON88017 with the established method was 5 copies at the 97.5% confidence level. Thus, the real-time fluorescent quantitative PCR assay established in this study exhibited high specificity, accuracy and sensitivity, which could provide technical support for the safety supervision of genetically modified organ- isms and products in China.

双重荧光实时定量PCR法检测TNF-α mRNA表达水平

目的:建立单管检测肿瘤坏死因子-α(TNF-α)和内参GAPDH mRNA表达水平的双重荧光实时定量PCR方法。方法:脂多糖刺激小鼠巨噬细胞Ana-1后提取细胞RNA,经反转录合成c DNA,应用自行设计的不同荧光标记的TNF-α和GAPDH引物探针,经PCR扩增后,在FAM通道和CY5通道分别读取Ct值,同时应用基因测序技术对结果进行验证,并构建质粒标准品分析该方法的灵敏度和重复性。结果:双重荧光实时定量PCR法检测TNF-α的灵敏度达4×101拷贝/μL,检测线性范围可达6个数量级,批内和批间重复性好。结论:新方法消除了目的基因与内参的加样误差,节约成本,快速准确,适用于TNF-αmRNA的定量检测。

双重TaqMan荧光定量PCR在β-地中海贫血产前诊断中的应用

目的建立基因点突变双重TaqMan荧光定量PCR方法,实现β-地中海贫血(β-地贫)高风险胎儿产前基因诊断快速、准确。方法以每反应管检测一个位点的突变和野生型基因序列,建立β-地贫基因点突变双重TaqMan荧光定量PCR体系,检测β-地贫高风险胎儿绒毛标本6例、羊水标本32例,根据荧光PCR阳性扩增结果结合两荧光通道的Ct值差异分析受检标本的基因型,同时以常规RDB检测为对照,分析与评价检测结果。结果 6例胎儿绒毛标本中,RDB检测无法判断结果 1例,经该方法检测为野合纯合子;RDB检测误诊为CD41-42合并CD26双重杂合子1例,经该方法检测为CD41-42杂合子。32例胎儿羊水标本中,RDB检测无法判断的标本1例,经该方法检测为CD41-42杂合子。该3例标本经重新采集胎儿羊水标本复查,验证了定量检测结果的准确性。结论β基因点突变双重TaqMan荧光PCR定量检测方法,可实现β-地贫高风险胎儿的快速准确产前基因诊断,操作简单快速,结果准确可靠,是较为理想的β-地贫产前诊断方法。

基于DPO引物检测猪流行性腹泻病毒荧光定量RT-PCR方法的建立及初步应用

为建立快速、准确检测猪流行性腹泻病毒(PEDV)的方法,本研究以PEDV的N基因为靶基因,基于双启动寡核苷酸引物(DPO),经过条件优化,建立了检测PEDV的荧光定量RT-PCR方法。结果显示,DPO引物的有效退火温度范围较宽(45℃~65℃);在测试的10种病毒中仅PEDV为阳性扩增结果,其余病毒为阴性结果,特异性较强;对PEDV质粒标准品的检测限可达1.64×10^1拷贝/μL,敏感性较高;组内、组间重复性结果的变异系数均小于1%,重复性较好。利用该方法对采集的272份临床仔猪腹泻样品(粪便、小肠组织)进行检测,结果显示,共检出PEDV阳性样品39份,阳性率为14.34%,与常规RT-PCR方法检测结果的阳性符合率为92.31%;本研究建立方法检测的阳性样品经PEDV N基因测序鉴定,确实均为PEDV阳性样品。本研究建立的基于DPO引物检测PEDV的荧光定量RT-PCR方法为PEDV的准确检测和流行病学调查提供技术支持。

染色体R显带分析、双色荧光原位杂交及实时荧光定量PCR对于急性早幼粒细胞性白血病诊断价值的评价

目的:评价染色体R显带技术(RT)、双色荧光原位杂交(D-FISH)和荧光定量PCR(RT-PCR)对急性早幼粒细胞白血病(APL)的诊断价值。方法:采用三种方法分析340例疑诊为APL患者的细胞遗传学特征或PML/RARa融合基因,以MICM综合诊断作为APL的诊断"标准",并与三者联合检测比较,评价RT、D-FISH和RT-PCR三者的诊断价值。结果:对于APL的诊断,RT、D-FISH以及RT-PCR三者的敏感度分别为81.3%(78/96),95.0%(91/96)和96.9%(93/96),RT漏检18例,D-FISH的检测结果判断5例假阳性,2例假阴性,RT-PCR的检测结果存在4例假阳性,3例假阴性。三者联合检测的敏感度为99.97%,特异度为100%。结论:三种检测方法单独应用于APL的诊断均存在一定的弊端,三者联合运用有利于提高临床诊断率,同时减少误诊率和漏诊率。

双重实时荧光定量PCR检测人维生素D受体的方法学构建

目的 建立单管检测人维生素D受体（VDR）及甘油醛-3-磷酸脱氢酶（GAPDH）基因的双重实时荧光定量聚合酶链反应（dual real-time PCR）的方法。方法 以GAPDH基因为内参,采用Primer Premier 5.0软件设计特异性引物及Taq Man探针,进行PCR扩增检测VDR基因。将VDR及GAPDH扩增产物片段纯化后克隆构建成重组质粒,作为定量检测基因表达的标准品,并用于分析该方法的灵敏度和重复性。结果 PCR扩增产物经测序分析证实为VDR及GAPDH特异性片段;该方法检测VDR与GAPDH灵敏度达40拷贝/μL;线性范围为4.00×10~1~4.00×10~5拷贝/μL;决定系数R2分别为0.998、0.999;扩增效率E分别为96.10%、85.15%;批内变异系数（CV）分别为0.09%~1.21%、0.35%~0.88%;批间CV分别为0.17%~0.51%、0.51%~2.46%。结论 成功建立了单管检测人VDR及GAPDH的双重实时荧光定量PCR方法,且该方法特异性好、灵敏度高、可快速高通量检测VDR的相对表达量,有效缩短时间,减小实验误差。

双重实时荧光定量PCR技术检测中药制剂中沙门氏菌和大肠埃希菌

目的:建立双重实时荧光定量PCR(multiplex quantitative real-time PCR,multiplex qPCR)快速检测中药制剂中沙门氏菌和大肠埃希菌2种常见控制菌的方法。方法:筛选两种目标菌株的特异性引物与探针,扩增沙门氏菌的invA基因和大肠埃希菌的uidA基因,优化反应体系,建立双重荧光定量PCR方法。结果:两对引物探针对沙门氏菌和大肠埃希菌均有较好地扩增效率,人工污染中药制剂中沙门氏菌的检出限为101 CFU·mL^(-1),大肠埃希菌的检出限为101 CFU·mL^(-1)。结论:本研究建立的双重实时荧光定量PCR方法具有特异性强、重复性好,灵敏度高等特点、适用于中药制剂中沙门氏菌和大肠埃希菌的快速检测。

沙眼衣原体、单纯疱疹病毒2型双重荧光定量PCR检测方法的建立

目的建立双重实时荧光定量PCR检测沙眼衣原体和单纯疱疹病毒2型的方法。方法针对沙眼衣原体和单纯疱疹病毒2型基因组保守序列,设计引物和探针,建立双重荧光定量PCR检测方法,评价其敏感性、特异性,并与常规单重荧光PCR方法比较。结果成功建立了双重实时荧光定量PCR检测沙眼衣原体和单纯疱疹病毒2型的方法,检测限均为1000copies/μL,敏感性和特异性均为100%。应用该方法检测了50份患者标本,与试剂公司提供的单重荧光PCR试剂检测结果一致性为100%。结论该研究建立的快速、准确,可同时检测沙眼衣原体、单纯疱疹病毒2型的双重实时荧光定量PCR法,具有较高的敏感性、特异性和稳定型,操作简单,可用于沙眼衣原体、单纯疱疹病毒2型的临床筛查和诊断。

6319例高危型人乳头瘤病毒核糖核酸定量检测的结果分析

目的探讨女性高危型人乳头瘤病毒(HPV)感染亚型分布情况及年龄特点。方法采用双通道实时荧光定量PCR检测方法,对6319例女性高危型HPV-DNA 16型、HPV-DNA 18/45型、HPV-DNA 31型、HPV-DNA 33/52/58/67型进行定量分析,比较不同年龄组HPV-DNA阳性率及不同型别HPV-DNA的分布。结果 6319例女性中检出HPV-DNA阳性患者794例,总阳性率为12.6%。51～60岁组与≥61岁组的阳性率均为15.8%,且高于其他年龄组差异有统计学意义(P<0.05),其次为21～30岁组阳性率为13.8%。不同类型HPV-DNA阳性率从高到低依次为HPV-DNA 33/52/58/67型(69.3%)、HPV-DNA 16型(21.5%)、HPV-DNA 18/45型(12.1%)、HPV-DNA 31型(6.9%)。结论高危型人乳头瘤病毒核糖核酸定量检测可用初筛女性宫颈癌的人群,更应作为年龄在38～58岁的女性健康体检时的必选项目,且对宫颈癌的诊断和药物治疗具有重要意义。

利用双萤光素酶报告基因系统筛选有效的siRNA

目的建立一种利用双萤光素酶报告基因系统筛选能有效抑制目的基因表达的小干扰RNA(siRNA)的方法。方法以绿色荧光蛋白(GFP)基因为研究对象,构建3个候选的靶向GFP的siRNA表达质粒pSi-GFPsiRNA1、pSi-GFPsiRNA2、pSi-GFPsiRNA3和阴性对照pSi-Negative。构建拥有同一Kozak共有翻译启始序列、翻译启始密码子ATG的GFP与萤光素酶基因(LUC)的融合表达载体pGL3-GFPf。将包含3个GFPsiRNA靶序列的GFP片段插入到改建过的pGL3-promoter载体上LUC的3'非翻译区(UTR),构建pGL3-GFPp。将GFPsiRNA表达质粒联同内参照质粒pRL-TK分别与pGL3-GFPf、pGL3-GFPp共转化HEK293细胞。利用双萤光素酶检测试剂盒测定各组细胞中萤光素酶的活力水平,用荧光定量PCR检测各组细胞中GFPmRNA的表达水平。结果同对照组相比,与pGL3-GFPf共转化GFPsiRNA表达质粒的各组细胞中萤火虫萤光素酶/海肾萤光素酶比值明显降低,其中GFPsiRNA1表达组中降低最显著(P<0.01);定量PCR检测也显示,GFPsiRNA1表达组中GFPmRNA的表达水平降低最明显(P<0.01)。双萤光素酶活性检测和定量PCR结果还显示,与pGL3-GFPp共转化GFPsiRNA表达质粒的各组细胞中,GFPsiRNA1抑制GFP的表达最显著(P<0.01)。结论本文建立了通过双萤光素酶活性检测来筛选有效的siRNA的方法,并为进行多个基因的有效siRNA的筛选提供解决方案。

狂犬病病毒和犬2型腺病毒双重荧光定量PCR检测方法的建立及应用

目的为了解CAV2-ΔE3-CGS口服疫苗免疫后排毒情况和掌握犬腺病毒(CAV)感染本底情况,研究建立狂犬病病毒和犬2型腺病毒双重荧光定量PCR检测方法。方法针对CAV2-ΔE3-CGS中犬2型腺病毒E1基因和狂犬病病毒G基因设计特异性引物和探针,建立检测CAV2-ΔE3-CGS的双重荧光定量PCR检测方法,并对实验动物场和犬类留验场流浪犬口鼻拭子和环境样本进行了检测。结果该方法生成的标准曲线分别为Y=-3.351×logX+44.895,R^(2)为0.999和Y=-3.413×logX+45.192,R^(2)为0.996,线性关系良好,最低检测线都为102拷贝/μL。在实验动物场流浪犬和环境中未检测到CAV2-ΔE3-CGS;在犬类留验场流浪犬中检测到CAV感染,其中口鼻拭子阳性率为5.88%(5/85),肛拭子阳性率为8.24%(7/85),环境样本阳性率为4.00%(1/25)。结论研究建立的双重荧光定量PCR检测方法适用于CAV2-ΔE3-CGS排毒情况排查和CAV感染调查。研究表明CAV2-ΔE3-CGS免疫后未检测到排毒,上海市流浪犬CAV感染率较低,因此符合CAV2-ΔE3-CGS的口服免疫要求。

Temperature Stress at Grain Filling Stage Mediates Expression of Three Isoform Genes Encoding Starch Branching Enzymes in Rice Endosperm

An early-maturity indica rice variety Zhefu 49, whose grain quality and starch structure are sensitive to environmental temperature, was subjected to different temperatures （32℃ for high temperature and 22℃ for optimum temperature） at the grain filling stage in plant growth chambers, and the different expressions of three isoform genes （SBEI, SBEIII and SBE/V） encoding starch branching enzyme （SBE） in the endosperms were studied by the real-time fluorescence quantitative PCR （FQ-PCR） method. Effects of high temperature on the SBE expression in developing rice endosperrns were isoform-dependent. High temperature significantly down-regulated the expressions of SBEI and SBEIII, while up-regulated the expression of SBEIV. Compared with SBEIV and SBEIII, the expression of SBEI gene in Zhefu 49 rice endosperms was more sensitive to temperature variation at the grain filling stage. This study indicates that changes in weather/climate conditions especially temperature stress influence rice grain formation and its quality as evidenced by isoform expression.

Expressions of Toll Like Receptor(TLR)Genes in Paralichthys olivaceus After Induced by Different Extracts of Edwardsiella tarda

Toll like receptors(TLRs)are the main innate immune‘pattern recognition receptors’of animals,which play a central role in host cell recognition and responses to invasive pathogens,particularly common structures of microbial pathogens.In this study,the gene expression profiles of TLRs in the spleen,head kidney,gill,small intestine,liver,muscle,and heart of healthy Paralichthys olivaceus were detected by real-time quantitative PCR(qPCR).The TLR family members were widely expressed in different tissues with different basic expression profiles.The highest expressions of TLR1,5m,7,8,9,14,and 21 were found in the spleen;the highest expressions of TLR3 and TLR21 were found in the gill;the highest expressions of TLR2 and 5s were found in the small intestine.The second highest expressions of TLR3,7,and 8 were found in small intestine.The gene expression profiles of TLRs stimulated with Edwardsiella tarda DNA,RNA,and lipopolysaccharide(LPS)were also detected in spleen,head kidney and gill.TLR9 and TLR21 were sensitive to E.tarda DNA;TLR 8 and TLR21 were sensitive to E.tarda RNA;and TLR1 and TLR14 were sensitive to E.tarda LPS.The expressions of the other TLR genes showed no significant changes.The results imply that the expressions of these TLR genes in P.olivaceus are differently regulated in the whole body and play important roles in the immune response against E.tarda infection.

A simple and visualized method to screen for effective siRNAs by using green fluorescence protein (GFP) as a reporter

To screen for effective small interference RNA(siRNA),a simple and visualized method was developed using the green fluorescence protein(GFP)as a reporter.Candidate siRNAs targeting macrophage migration inhibition factor genes(MIF)were identified.By using the pEGFP-N3 vector,the MIF-GFP expression plasmid,pEGFP-MIF,was constructed with the same Kozak consensus translation initiation site and start code ATG for the MIF-EGFP coding sequence.Based on the siRNA expression vector pSilencer-4.1,3 candidate MIF siRNA expression plasmids were constructed and co-transfected with the pEGFP-MIF into the HEK293 cells,respectively.The GFP expression in HEK293 cells could be viewed by fluorescence microscopy and the MIF mRNA expressions were determined by real-time quantitative PCR.The 3 candidate MIF siRNA expression plasmids were also co-transfected with the MIF expression plasmid into the HEK293 cells,respectively,and the MIF mRNA expressions were determined by real-time quantitative PCR.The results show that the down-regulated expression of the MIF mRNA was consistent with the GFP expression and the same effective MIF siRNAs were screened by using the pEGFP-MIF or MIF expression plasmid with the candidate MIF siRNAs expression plasmids.Therefore,by using the GFP as a reporter,a useful method was provided to screen for effective siRNAs targeting specific genes co-expressed with the GFP.This may be a good strategy for screening for effective siRNAs targeting different genes.

Developmental Changes of GH Gene in Tan Sheep and Correlation Analysis with Slaughter Traits

[ Objective] The paper was to study the differential expression of growth hormone （GH） gene in different ages and different tissues of Tan sheep. [ Method] Using real-time fluorescent quantitative PCR （RT-PCR） assay, specific primers were designed according to the GH gene sequence published on Gen- Bank. With the total RNA of Tan sheep tissue as the template, the expression levels of GH gene in pectoral muscle, leg muscle and longissimus dorsi muscle at dif- ferent ages were analyzed. [ Result] In three types of muscle tissues, the expression patterns of GH gene in different tissues at the same month of age were pectoral muscle 〉 leg muscle 〉 longissimus dorsi muscle. The expression levels of GH gene were positively correlated with live weight before slaughter, carcass weight and net meat weight, and had significant positive correlation only with net meat weight （ P 〈 0.05 ）. [ Conclusion ] The content of GH gene in different tissues gradually increased with the increasing months of age, and there were extremely significant differences in expression level of GH gene among different months of age or different sites （P〈0. 01）.