FQ-PCR与血清型特异性抗体法检测HSV-2的临床意义

目的分析荧光定量聚合酶链反应(FQ-PCR)与血清型特异性抗体法对单纯疱疹病毒2型(HSV-2)的检测情况及其临床意义。方法对322例拟诊的生殖器疱疹患者分别采用FQ-PCR与HSV-2血清型特异性抗体2种方法进行HSV-2检测,并对其检测结果及临床特征进行统计学分析。结果 322例拟诊生殖器疱疹患者FQ-PCR共检出HSV-2阳性148例,阳性率为45.96%;不同类型临床标本FQ-PCR阳性率有明显差异,其中水疱液的检出率最高,为60.26%,溃疡/糜烂拭子的检出率为51.82%,结痂痂皮的检出率为17.85%。HSV-2血清型特异性抗体法共检出任一抗体阳性153例(占47.51%);HSV-2 IgG单一阳性133例(占36.74%);HSV-2 IgM单一阳性10例(占2.76%);IgG和IgM均阳性10例(占2.76%)。FQ-PCR和HSV-2 IgG两者单一阳性的病例比较后发现,FQ-PCR单一阳性病例其发病至检测时间[(4.36±3.80)d]少于HSV-2 IgG单一阳性病例[(9.27±7.25)d](P<0.01)。结论 FQ-PCR与血清型特异性抗体法同时检测有助于HSV-2感染的诊断。

S.Heidelberg血清型特异性基因筛选及PCR检测方法的建立与应用

海德尔堡沙门氏菌(Salmonella enterica serovar Heidelberg,SH)是沙门氏菌属内重要的致病性血清型。通过对SH基因组序列进行BLAST比对和PCR验证,筛选出了4个SH血清型特异性基因(SeHA_C2639、SeHA_C2640、SeHA_C3259和SeHA_C3258)。以SeHA_C3258作为靶点设计引物pHAm8(350bp)和沙门氏菌属特异性引物139-141(284bp),建立SH的PCR检测方法,并对其应用效果进行评价。结果表明,经55株不同血清型的沙门氏菌和其他常见食源性致病菌证明,该检测体系具有较好的特异性,纯菌菌落灵敏度为6.1×10~2 CFU/mL。以浓度为N×10~5~N×10~1 CFU/mL的大肠杆菌或鼠伤寒沙门氏菌为干扰菌时,该体系对10~2 CFU/mL的SH检测结果无影响。人工污染SH的牛奶样品,经8h培养,检测限达1.52CFU/mL。该检测方法能快速、准确检测出食品中的SH,有利于在食品安全领域中的应用。

甲型副伤寒沙门菌特异性基因筛选及PCR检测体系建立

以甲型副伤寒沙门菌为检测目标,通过比较基因组和聚合酶链式反应(polymerase chain reaction,PCR)验证方法筛选到4个该血清型的特异性基因,其中以gene_3105作为该血清型的检测靶点设计引物PA23;并结合沙门菌属特异性引物139-141,建立一种甲型副伤寒沙门菌的PCR检测方法。优化PCR反应体系,并对该检测体系的特异性、灵敏度、抗干扰能力及人工污染样品检出限等方面进行评价。结果表明,当样品中含有甲型副伤寒沙门菌时,该体系能扩增出2条特异性条带,含有其他血清型的沙门菌仅能扩增出284 bp条带,不含沙门菌无扩增条带产生。灵敏度评价表明,基因组DNA和纯菌菌落检出限分别为32.4 pg/μL和4.3×10~3 CFU/m L;抗干扰能力实验显示,当鸡肉背景菌群和猪肉背景菌群浓度在10~6 CFU/m L和4.87×10~7 CFU/m L时,检出限为6.43×10~4 CFU/m L。当无菌的鸡肉和猪肉样品中添加N CFU/25 g甲型副伤寒沙门菌时,经10 h增菌,检测结果为阳性(0<N<10)。实验建立甲型副伤寒沙门菌PCR检测方法具有较好的特异性和灵敏度,有很好的应用价值,可在食品安全领域广泛应用。

德尔卑沙门氏菌血清型分子检测靶点筛选及多重PCR检测方法的建立

利用比较基因组技术筛选到德尔卑沙门氏菌(Salmonella Derby, SD)的血清型特异性基因,以此为靶点设计引物与139-141引物共同构建多重PCR检测体系,对其特异性、菌落灵敏度、抗干扰能力及人工污染等方面进行评价。当扩增出171、284和512 bp电泳条带时,检测结果为阳性。通过该方法检测39株沙门氏菌和18株非沙门氏菌,表现出100%特异性,该检测体系的DNA灵敏度为383.2 pg/μL,菌落灵敏度为52 CFU/mL。当SD与自然(猪肉、鸡肉和牛肉)的背景菌群浓度比为1∶10~4时,该检测体系能获得清晰、准确的3条扩增条带。在人工污染的猪肉、鸡肉和牛肉样品的检测中,增菌10 h,检测灵敏度为3.8 CFU/25g。该检测方法准确灵敏的检测SD,可在食品安全领域得到广泛应用。

肺炎链球菌型特异性IgG抗体定量ELISA方法建立与验证

目的建立WHO推荐的肺炎链球菌血清型特异性IgG抗体定量ELISA检测方法。方法参照WHO Pn PS ELISA操作手册,采用ATCC来源肺炎链球菌荚膜多糖4、6B、9V、14、18C、19F、23F型为包被抗原,以007sp为标准血清建立本实验室的人血清中肺炎链球菌血清型特异性IgG抗体定量ELISA检测方法。并用WHO校准血清盘(12/278)和内部质控血清PnG对所建方法准确性、稳定性进行验证。结果确定了4、6B、9V、14、18C、19F、23F共7个血清型荚膜多糖的抗原包被浓度;建立了适用于本实验室的人血清中肺炎链球菌血清型特异性IgG抗体定量ELISA检测方法。12份WHO校准血清的验证结果显示,所测7个血清型IgG抗体中,均有>75%的检测值落在WHO参比实验室赋值的±40%范围之内,总符合率达到86.9%,相关性曲线斜率(slope)=0.94,R2=0.99,达到了WHO规定的室间评价要求。此外,连续20次的内部质控血清PnG的检测结果显示,不同批次检测值的变异系数(CV)均≤15%,达到了WHO规定的室内评价要求。结论本实验室成功建立WHO推荐的检测人血清中肺炎链球菌血清型特异性IgG抗体定量ELISA检测方法,并经验证所建方法结果准确,方法稳定,具备了开展疾病监测与疫苗效果评价应用要求。

慢性肺部疾病患者接种23价肺炎链球菌多糖疫苗后抗荚膜多糖抗体的特异性

目的探讨慢性肺部疾病患者接种23价肺炎链球菌多糖疫苗(PPV)后血清中抗肺炎链球菌荚膜多糖(CPS)IgG抗体的特异性。方法以39例慢性肺部疾病患者为研究对象,分别用第二代和特异性更高的第三代ELISA测定疫苗接种前、后血清中的肺炎链球菌6B、19F和23F三种血清型的特异性IgG抗体浓度。结果用第三代ELISA测得的患者血清中血清型特异性IgG抗体水平比用第二代ELISA测得的抗体水平显著降低。无论是PPV接种前的自然感染,还是PPV接种后的主动免疫,慢性肺部疾病患者血中产生的抗CPS-IgG中都有大约一半的非特异性抗体。结论 PPV接种并不能提高慢性肺部疾病患者血中的特异性抗CPS-IgG的比例。

Comparison of Multiplex Fluorescent PCR with Serum Type-specific Antibody Detection in Diagnosis of Genital Herpes

Objectives: To compare multiplex fluorescent PCRwith serum type-specific antibody detection in thediagnosis of herpes simplex virus (HSV) infection andto evaluate its significance in the diagnosis of genitalherpes.Methods: We detected HSV infection in 121 speci-mens collected from patients with genital herpesusing both multiplex fluorescent PCR and serum type-specific antibody detection. HSV viral isolation wasused as the standard control.Results: When compared with the viral isolation, thesensitivity and specificity for multiplex fluorescentPCR were 100% and 88.89%, respectively afterdiscrepant analysis. The sensitivity and specificity fortype-specific antibody detection was 77.68 % and77.78 %, respectively. However, the type-specificantibody detected HSV in two asymptomatic patientswhile the multiplex fluorescent PCR couldn’t detectany HSV DNA from those specimens.Conclusions: Multiplex fluorescent PCR is a verysensitive and specific method for detection and typingof HSV in the lesion of genital herpes, it failed todetect HSV DNA from the asymptomatic patients.Serum type-specific antibody detection was a lesssensitive and specific test but could detect the specificantibody from some asymptomatic patients. Thecombination of these two techniques would allow rapid,sensitive and accurate detection and typing of HSVand help clinical diagnosis and epidemiologic survey-ing of genital herpes.

Establishment of a transgenic mouse model with liver-specific expression of secretory immunoglobulin D

Mutation of mevalonate kinase （MVK） is thought to account for most cases of hyperimmunoglobulinemia D syndrome （HIDS） with recurrent fever. However, its mechanism and the relationship between elevated serum immunoglobulin D （IgD） and the clinical features of HIDS are unclear. In this study, we generated by fusion PCR a vector to express high levels of chimeric secretory IgD （cslgD） specifically in the liver. We then generated seven founder lines of transgenic mice by co-microinjection, and verified them using genomic PCR and Southern blotting. We detected the expression of csIgD by reverse transcription PCR, quantitative PCR, western blotting, and enzyme-linked immunosorbent assays. We demonstrated that csIgD could be specifically and stably expressed in the liver. We used flow cytometry to show that overexpression of csIgD in the bone marrow and spleen cells had no effect on B cell development. Morphologic and anatomical observation of the transgenic mice revealed skin damage, hepatosplenomegaly, and nephromegaly in some transgenic mice; in these mice, pathological sections showed high levels of cell necrosis and protein-like sediments in the liver, spleen, and kidney. We demonstrated that the genomic insertion sites of the transgeues did not disrupt the MVK gene on mouse chromosome 5. This transgenic mouse will be useful to explore the pathogenesis of HIDS.