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2型腺病毒有效感染后期的基因组表达与mRNA成熟

Genome expression and mRNA maturation at late stages of productive adenovirus type 2 infection.

作者信息

Wold W S, Green M, Brackmann K H, Cartas M A, Devine C

出版信息

J Virol. 1976 Nov;20(2):465-77. doi: 10.1128/JVI.20.2.465-477.1976.

Abstract

RNA from adenovirus 2-infected KB cells was annealed in liquid with RNA in vast excess to viral heavy (l) and light (r) 32P-labeled DNA strands. Hybridization kinetics were analyzed by computer to estimate the number of viral RNA abundance classes, their relative concentrations, and the fraction of each DNA strand from which they originated. Early whole cell RNA extracted 5 h postinfection annealed rapidly to 10 to 15% of l and r strands and then slowly to final values of 60 and 40% of l and r strands. By 9 h postinfection the expression of late genes was apparent and whole cell RNA annealed to 20 and 75% of l and r strands. Whole cell RNA extracted between 12 and 36 h postinfection annealed to 7 to 15% and 75 to 90% of l and r strands. Late nuclear RNA hybridized to 10 and 90% of l and r strands, and late polyribosomal RNA hybridized to 20 and 75% of l and r strands. Based upon kinetic analyses, we estimate that mRNA synthesized exclusively during late stages arises from about 6 to 8% and 45 to 49% of l and r strands. This assumes that the early class I mRNA (in low concentration late) originates from 8 to 10% and 6 to 10% of l and r strands and that early class II mRNA (in high concentration late) is derived from 2% and 8 to 13% of l and r strands. Mixing experiments indicated that early mRNA is a subset of RNA extracted from polyribosomes late after infection and that late nuclear RNA contains sequences complementary to early l strand class I nRNA. RNA-RNA hybrids were isolated from late mRNA containing sequences from 60% of l and r strands, but it is not known when these were synthesized, and therefore whether complementary RNA transcripts are synthesized late after infection, as they are known to be synthesized early. These results demonstrate that portions of the genome are transcribed into RNA sequences that remain confined to the nucleus and are not exported to polyribosomes as mRNA.

摘要

来自腺病毒2感染的KB细胞的RNA与大量过量的RNA在液体中退火,该过量RNA与病毒重链(l)和轻链(r)32P标记的DNA链结合。通过计算机分析杂交动力学,以估计病毒RNA丰度类别的数量、它们的相对浓度以及它们所源自的每条DNA链的比例。感染后5小时提取的早期全细胞RNA迅速退火至l链和r链的10%至15%,然后缓慢退火至l链和r链最终值的60%和40%。到感染后9小时,晚期基因的表达明显,全细胞RNA退火至l链和r链的20%和75%。感染后12至36小时提取的全细胞RNA退火至l链和r链的7%至15%和75%至90%。晚期核RNA与l链和r链的10%和90%杂交,晚期多核糖体RNA与l链和r链的20%和75%杂交。基于动力学分析,我们估计仅在晚期阶段合成的mRNA分别来自l链和r链的约6%至8%和45%至49%。这假设早期I类mRNA(晚期浓度低)分别来自l链和r链的8%至10%和6%至10%,并且早期II类mRNA(晚期浓度高)分别来自l链和r链的2%和8%至13%。混合实验表明,早期mRNA是感染后期从多核糖体中提取的RNA的一个子集,并且晚期核RNA包含与早期l链I类nRNA互补的序列。从包含l链和r链60%序列的晚期mRNA中分离出RNA-RNA杂交体,但不知道这些杂交体何时合成,因此也不知道互补RNA转录本是否像已知在早期合成那样在感染后期合成。这些结果表明,基因组的部分被转录成RNA序列,这些序列仍局限于细胞核内,不会作为mRNA输出到多核糖体。

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