通过逆转录聚合酶链反应(RT-PCR)从粪便标本中扩增人B组轮状病毒的各种基因。
Amplification of various genes of human group B rotavirus from stool specimens by RT-PCR.
作者信息
Sen A, Kobayashi N, Das S, Krishnan T, Bhattacharya S K, Urasawa S, Naik T N
机构信息
Division of Virology, National Institute of Cholera and Enteric Diseases, P-33, C.I.T. Road, Scheme XM, Beliaghata, 700 010, Calcutta, India.
出版信息
J Clin Virol. 2000 Sep 1;17(3):177-81. doi: 10.1016/s1386-6532(00)00093-7.
BACKGROUND
The detection of the human group B rotavirus (HuGBR) CAL strain from India has given us an opportunity to design suitable primers for the detection of HuGBR since CAL is the second HuGBR detected until now, the Chinese Adult Diarrhoea Rotavirus (ADRV) being the first reported human pathogen belonging to this group of viruses. The primers described here may thus be used for the detection of human group B rotaviruses by reverse transcription-PCR (RT-PCR) in a diagnostic laboratory.
OBJECTIVE
To establish a set of primers suitable for the detection of various genes of human group B rotaviruses using a rapid RT-PCR assay.
STUDY DESIGN
Until recently, the Chinese ADRV strain was the only HuGBR strain that had been partially sequenced by cloning various viral genes using vector-specific primers. Consequently, there are very few reports in the literature describing primers that may be used for the detection of HuGBR viruses using RT-PCR in a clinical laboratory. The sequences of various genes from the ADRV strain that had been submitted to the nucleotide sequence database GenBank were analyzed in order to design several putative detection primer pairs for an RT-PCR assay. The rationale was to amplify the cognate genes from five isolates of the HuGBR CAL strain (CAL-1 to CAL-5) that have been detected to date from India. Primers that resulted in a specific product of the expected size from the CAL isolates were used to standardize a protocol for amplifying various genes of the CAL isolates under identical reaction conditions.
RESULTS
Out of several synthetic oligonucleotides designed, 12 were found to be satisfactory for the amplification of gene segments 4, 5, 6, 7, and 9 from the five CAL isolates and are presented here. A set of previously described primers that have been shown to be specific for human group B rotavirus gene segment 8 were also found to amplify the cognate gene from the CAL isolates. All the reactions were carried out using the same thermal cycling conditions.
CONCLUSIONS
The extreme virulence potential of HuGBR has been documented in several epidemics in China. Until recently, the Chinese ADRV strain was the only known HuGBr strain. As there have not been any reports of HuGBR infections outside China, there are no consensus nucleotide sequences available for HuGBR that may be used to validate primers for the detection of HuGBR. Here we report a set of 12 primer sequences that were designed from ADRV sequences and also found to amplify various genes from the different CAL isolates and hence may represent consensus primers suitable for the detection of HuGBR.
背景
从印度检测到的人B组轮状病毒(HuGBR)CAL株,为我们设计检测HuGBR的合适引物提供了契机,因为CAL是迄今为止检测到的第二株HuGBR,中国成人腹泻轮状病毒(ADRV)是首个被报道的属于该病毒组的人类病原体。因此,这里描述的引物可用于诊断实验室通过逆转录聚合酶链反应(RT-PCR)检测人B组轮状病毒。
目的
使用快速RT-PCR检测法建立一套适合检测人B组轮状病毒各种基因的引物。
研究设计
直到最近,中国ADRV株是唯一一株通过使用载体特异性引物克隆各种病毒基因而进行了部分测序的HuGBR株。因此,文献中很少有描述可用于临床实验室通过RT-PCR检测HuGBR病毒的引物的报道。分析了已提交到核苷酸序列数据库GenBank的ADRV株各种基因的序列,以便为RT-PCR检测设计几个假定的检测引物对。基本原理是从迄今已从印度检测到的HuGBR CAL株的五个分离株(CAL-1至CAL-5)中扩增同源基因。从CAL分离株中产生预期大小特异性产物的引物用于标准化在相同反应条件下扩增CAL分离株各种基因的方案。
结果
在设计的几种合成寡核苷酸中,发现12种对于从五个CAL分离株中扩增基因片段4、5、6、7和9是令人满意的,在此展示。还发现一组先前描述的对人B组轮状病毒基因片段8具有特异性的引物也能从CAL分离株中扩增同源基因。所有反应均在相同的热循环条件下进行。
结论
HuGBR的极高毒力潜能已在中国的几次疫情中得到记录。直到最近,中国ADRV株是唯一已知的HuGBR株。由于在中国境外尚无HuGBR感染的报道,因此没有可用于验证检测HuGBR引物的HuGBR一致核苷酸序列。在此,我们报告了一组12个引物序列,这些序列是根据ADRV序列设计的,并且也能从不同的CAL分离株中扩增各种基因,因此可能代表适合检测HuGBR的一致引物。
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