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基因46和47在噬菌体T4繁殖中的作用。I. 体内脱氧核糖核酸复制

Role of genes 46 and 47 in bacteriophage T4 reproduction. I. In vivo deoxyribonucleic acid replication.

作者信息

Hosoda J, Mathews E, Jansen B

出版信息

J Virol. 1971 Oct;8(4):372-87. doi: 10.1128/JVI.8.4.372-387.1971.

Abstract

Functional proteins coded by genes 46 and 47 are required for (i) continuation of deoxyribonucleic acid (DNA) synthesis in the late period of T4 infection and (ii) production of normal, late replicating DNA which contains strands with a sedimentation coefficient in alkaline sucrose greater than that of mature DNA (73S). Continued DNA synthesis in the late period in the absence of functional genes 46 or 47 can be achieved by inhibiting late protein synthesis either by using bacterio-phage with a second mutation in gene 55 or by adding chloramphenicol to the culture before the decline in the rate of DNA synthesis. However, when functional 46/47 proteins are absent throughout infection, no strands with a sedimentation coefficient greater than 73S (in alkaline sucrose) are produced. This is the case even when DNA synthesis is allowed to continue. DNA arrest is accompanied by conversion of rapidly sedimenting, replicating DNA to slower sedimenting forms. When 46/47 is absent from the beginning of infection, the conversion product has a smaller sedimentation coefficient than mature DNA both in neutral and alkaline sucrose. When DNA arrest occurs midway in infection by heat-inactivating the ts46 enzyme, the conversion product has a sedimentation coefficient (i) the same as mature DNA in both neutral (63S) and alkaline sucrose if capsid assembly is allowed to take place and (ii) close to 63S in neutral sucrose but heterogenous and relatively greater (up to 100S) in alkaline sucrose if capsid assembly is inhibited. The structure of this DNA is unknown.

摘要

基因46和47编码的功能蛋白对于以下两点是必需的:(i)在T4感染后期脱氧核糖核酸(DNA)合成的继续;(ii)产生正常的、后期复制的DNA,其包含在碱性蔗糖中沉降系数大于成熟DNA(73S)的链。在缺乏功能基因46或47的情况下,后期DNA合成的继续可以通过以下方式实现:使用在基因55中有第二个突变的噬菌体,或者在DNA合成速率下降之前向培养物中添加氯霉素来抑制后期蛋白质合成。然而,当在整个感染过程中缺乏功能性的46/47蛋白时,不会产生沉降系数大于73S(在碱性蔗糖中)的链。即使允许DNA合成继续,情况也是如此。DNA停滞伴随着快速沉降的复制性DNA向沉降较慢形式的转变。当从感染开始就缺乏46/47时,在中性和碱性蔗糖中,转变产物的沉降系数都比成熟DNA小。当通过热灭活ts46酶在感染中期发生DNA停滞时,如果允许衣壳组装,转变产物的沉降系数(i)在中性(63S)和碱性蔗糖中都与成熟DNA相同;(ii)如果衣壳组装受到抑制,在中性蔗糖中接近63S,但在碱性蔗糖中是异质的且相对更大(高达100S)。这种DNA的结构尚不清楚。

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SEDIMENTATION STUDIES OF THE SIZE AND SHAPE OF DNA.DNA大小与形状的沉降研究
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