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通过原位杂交检测腺病毒转化细胞中的病毒DNA序列。

Detection of viral DNA sequences in adenovirus-transformed cells by in situ hybridization.

作者信息

Loni M C, Green M

出版信息

J Virol. 1973 Dec;12(6):1288-92. doi: 10.1128/JVI.12.6.1288-1292.1973.

Abstract

Cytological preparations of cells transformed by members of three groups of human adenoviruses, adenovirus 12, 7, and 2, were annealed with radioactive complementary RNA (cRNA) (4 x 10(7) to 4.5 x 10(7) dpm/mug) prepared by copying viral DNA with the Escherichia coli DNA-directed RNA polymerase. These in situ hybridizations detected adenovirus-specific DNA sequences in interphase nuclei when transformed cells were annealed with homologous viral cRNA, but not with heterologous viral cRNA. The highest autoradiographic grain counts were found over adenovirus 7-transformed cell nuclei, next over adenovirus 12-, and the lowest over adenovirus 2-transformed cell nuclei. This is the same order as found by reassociation kinetic measurements (K. Fujinaga and M. Green, unpublished data).

摘要

用三组人类腺病毒(腺病毒12型、7型和2型)成员转化的细胞的细胞学制剂,与通过用大肠杆菌DNA指导的RNA聚合酶复制病毒DNA制备的放射性互补RNA(cRNA)(4×10⁷至4.5×10⁷ dpm/μg)进行退火处理。当用同源病毒cRNA而不是异源病毒cRNA对转化细胞进行退火处理时,这些原位杂交在间期核中检测到腺病毒特异性DNA序列。在腺病毒7转化的细胞核上发现最高的放射自显影颗粒计数,其次是腺病毒12转化的细胞核,而在腺病毒2转化的细胞核上最低。这与通过重缔合动力学测量发现的顺序相同(藤永健和格林,未发表数据)。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/88fa/356770/c279a80da8e4/jvirol00264-0112-a.jpg

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