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单纯疱疹病毒1型基因US11的产物作为一个真正的晚期基因表达。

The product of gene US11 of herpes simplex virus type 1 is expressed as a true late gene.

作者信息

Johnson P A, MacLean C, Marsden H S, Dalziel R G, Everett R D

出版信息

J Gen Virol. 1986 May;67 ( Pt 5):871-83. doi: 10.1099/0022-1317-67-5-871.

Abstract

The genes of herpes simplex virus type 1 (HSV-1) can be divided into at least three temporally regulated groups termed immediate early (IE), early and late. We have studied in detail the expression of a member of the late class of genes, US11, which encodes a polypeptide of apparent molecular weight 21K. Highly specific and sensitive probes were used to monitor US11 RNA and protein synthesis during HSV-1 infection of tissue culture cells in the presence and absence of phosphonoacetic acid, an inhibitor of viral DNA replication. The results were compared with a similar study of the products of a delayed early gene, US6, encoding glycoprotein D (gD). It was found that the patterns of RNA and protein synthesis from US11 were significantly different to those of gD. US11 products appeared later and accumulated until late in infection, while gD RNA was significantly reduced at late times. In the presence of the inhibitor of DNA synthesis, US11 gene expression was reduced 50- to 100-fold while gD expression was reduced five- to tenfold. We conclude that US11 behaves as a true late gene during HSV-1 infection. However, the use of sensitive assays, which allowed the detection of very low levels of US11 gene products under conditions designed to eliminate DNA replication, brings into question the absolute requirement for DNA replication for the expression of a true late HSV-1 gene. These results are discussed in terms of current models for the regulation of late gene expression.

摘要

单纯疱疹病毒1型(HSV-1)的基因可至少分为三个受时间调控的组,即立即早期(IE)、早期和晚期。我们详细研究了晚期基因类成员US11的表达,该基因编码一种表观分子量为21K的多肽。在有和没有病毒DNA复制抑制剂膦甲酸的情况下,使用高度特异性和灵敏的探针来监测组织培养细胞在HSV-1感染期间US11 RNA和蛋白质的合成。将结果与对编码糖蛋白D(gD)的延迟早期基因US6产物的类似研究进行比较。发现US11的RNA和蛋白质合成模式与gD的明显不同。US11产物出现较晚,并积累至感染后期,而gD RNA在后期显著减少。在存在DNA合成抑制剂的情况下,US11基因表达降低了50至100倍,而gD表达降低了5至10倍。我们得出结论,在HSV-1感染期间,US11表现为一个真正的晚期基因。然而,使用灵敏的检测方法,在旨在消除DNA复制的条件下能够检测到极低水平的US11基因产物,这使得对于真正的HSV-1晚期基因表达是否绝对需要DNA复制产生了疑问。根据目前晚期基因表达调控模型对这些结果进行了讨论。

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