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通过对实验室菌株以及来自霍奇金淋巴瘤和骨髓移植患者的病毒变体进行序列分析,鉴定出两组人类疱疹病毒6型。

Two groups of human herpesvirus 6 identified by sequence analyses of laboratory strains and variants from Hodgkin's lymphoma and bone marrow transplant patients.

作者信息

Gompels U A, Carrigan D R, Carss A L, Arno J

机构信息

University of Cambridge Department of Medicine, Addenbrooke's Hospital, U.K.

出版信息

J Gen Virol. 1993 Apr;74 ( Pt 4):613-22. doi: 10.1099/0022-1317-74-4-613.

Abstract

Fifteen human herpesvirus 6 (HHV-6) strain variants were analysed by PCR amplifications, restriction enzyme site polymorphism and sequence analyses. Three DNA regions were chosen for study: a fragment of a variable glycoprotein gene (210 bp), the conserved glycoprotein H (gH) gene complete with intergenic sequences (2381 bp) and the 5' intergenic region with the N-terminal coding sequence of gH up to a polymorphic BamHI site (427 bp). Infected cell DNA from five laboratory reference strains including GS, U1102, AJ, Z29 and KF were examined together with DNA from peripheral blood lymphocytes infected with HHV-6 reactivated from blood and/or marrow from five bone marrow transplant (BMT) patients. Separate blood and marrow isolates were obtained from four BMT patients. In addition, HHV-6 sequences were examined directly from one of six Hodgkin's lymphomas and six B cell proliferations which contained HHV-6 DNA as detected by PCR amplification. The results show two groups of very closely related but heterogeneous strains which correlate with previous groupings by antigenic and restriction site differences. These are variant A strains (including laboratory strains GS, U1102 and AJ) and variant B strains (including laboratory strains Z29 and KF, the Hodgkin's lymphoma strain, and the nine BMT patient isolates). Variations between the groups were 4 to 6% in nucleotide sequence and 5 to 8.5% in amino acid sequence. Within each group maximum heterogeneity was observed in different genes. Variant A strains differed by 2.0% in the variable glycoprotein gene sequence whereas variant B strains were identical in this region; conversely, variant B strains differed by 2 to 3% in the gH N-terminal and intergenic sequences whereas variant A strains differed there by less than 0.2%. There was evidence for sequence drift independent of selection: relationships between the groups were shown by analyses of amino acid sequence, coding nucleotide sequence as well as intergenic sequence, and the B variant-specific BamHI site in the gH gene was due to a non-coding nucleotide substitution. There was little evidence for in vivo or in vitro variation: the gH nucleotide sequence from the uncultured lymphoma strain (first variant B gH gene identified) was almost identical to the gH sequence from four BMT isolates, and matched BMT isolates from blood and marrow were identical or with a single nucleotide substitution.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

通过聚合酶链反应(PCR)扩增、限制性酶切位点多态性分析及序列分析,对15株人疱疹病毒6型(HHV - 6)毒株变异体进行了分析。选取了三个DNA区域进行研究:一个可变糖蛋白基因片段(210 bp)、包含基因间序列的保守糖蛋白H(gH)基因(2381 bp)以及gH基因N端编码序列至多态性BamHI位点的5'基因间区域(427 bp)。对来自包括GS、U1102、AJ、Z29和KF在内的五株实验室参考毒株的感染细胞DNA,以及来自五名骨髓移植(BMT)患者血液和/或骨髓中重新激活的HHV - 6感染的外周血淋巴细胞DNA进行了检测。从四名BMT患者中分别获得了血液和骨髓分离株。此外,直接对六例霍奇金淋巴瘤中的一例以及六例B细胞增殖中的HHV - 6序列进行了检测,这些样本经PCR扩增检测含有HHV - 6 DNA。结果显示出两组密切相关但不同的毒株,这与先前根据抗原和限制性位点差异进行的分组相关。这些是A变异株(包括实验室毒株GS、U1102和AJ)和B变异株(包括实验室毒株Z29和KF、霍奇金淋巴瘤毒株以及九例BMT患者分离株)。两组之间的核苷酸序列差异为4%至6%,氨基酸序列差异为5%至8.5%。在每组内,不同基因中观察到最大异质性。A变异株在可变糖蛋白基因序列上的差异为2.0%,而B变异株在该区域相同;相反,B变异株在gH基因N端和基因间序列上的差异为2%至3%,而A变异株在该区域的差异小于0.2%。有证据表明序列漂移与选择无关:通过氨基酸序列、编码核苷酸序列以及基因间序列分析显示了两组之间的关系,并且gH基因中B变异株特异性的BamHI位点是由于非编码核苷酸取代所致。几乎没有证据表明存在体内或体外变异:未培养的淋巴瘤毒株(鉴定出的首个B变异株gH基因)的gH核苷酸序列与四例BMT分离株的gH序列几乎相同,并且来自血液和骨髓的匹配BMT分离株相同或仅有一个核苷酸取代。(摘要截断于400字)

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