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影响BK病毒游离型载体在人细胞中扩增的因素。简报。

Factors affecting amplification of BK virus episomal vectors in human cells. Brief report.

作者信息

Grossi M P, Caputo A, Paolini L, Balboni P G, Gerna G, Pagnani M, Corallini A, Barbanti-Brodano G

机构信息

Institute of Microbiology, School of Medicine, University of Ferrara, Italy.

出版信息

Arch Virol. 1988;99(3-4):249-59. doi: 10.1007/BF01311074.

Abstract

Analysis of factors determining replication of BK virus (BKV) episomal vectors in human cells showed that vector copy number was related to the level of BKV T antigen expression. T antigen was synthesized efficiently, as assessed by indirect immunofluorescence, in vector-transfected primary embryonic fibroblasts undergoing neoplastic transformation. Surprisingly, transfected continuous cell lines (143 B, HeLa and KB), kept under biochemical selection or tested in transient assays, produced negligible amounts or no T antigen, revealed only by a sensitive ELISA test, suggesting that in these cells vector amplification was under the control of cellular factors. Presence or absence of BKV late region sequences, BKV strain, orientation of the inserted genes and presence or absence of selection were not relevant for vector replication. Type of biochemical selection, however, was important, since BKV vectors containing the thymidine kinase gene replicated better than those containing the neo gene. Despite great variability, vector copy number increased in transfected clones of adenovirus 5-transformed 293 cells, in the absence of immunofluorescence detectable T antigen. These cells express adenovirus immediate early proteins E1A and E1B which may directly or indirectly activate BKV origin of replication.

摘要

对决定BK病毒(BKV)游离型载体在人细胞中复制的因素进行分析表明,载体拷贝数与BKV T抗原的表达水平相关。通过间接免疫荧光评估,在经历肿瘤转化的载体转染的原代胚胎成纤维细胞中,T抗原能高效合成。令人惊讶的是,在进行生化选择或瞬时检测时,转染的连续细胞系(143B、HeLa和KB)产生的T抗原量极少或不产生,只有通过灵敏的ELISA检测才能发现,这表明在这些细胞中载体扩增受细胞因子控制。BKV晚期区域序列的有无、BKV毒株、插入基因的方向以及选择的有无与载体复制无关。然而,生化选择的类型很重要,因为含有胸苷激酶基因的BKV载体比含有neo基因的载体复制得更好。尽管存在很大差异,但在没有免疫荧光可检测到的T抗原的情况下,腺病毒5转化的293细胞的转染克隆中载体拷贝数增加。这些细胞表达腺病毒立即早期蛋白E1A和E1B,它们可能直接或间接激活BKV复制起点。

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