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与血链球菌结合的同种转化DNA的命运

Fate of homospecific transforming DNA bound to Streptococcus sanguis.

作者信息

Raina J L, Ravin A W

出版信息

J Bacteriol. 1978 Mar;133(3):1212-23. doi: 10.1128/jb.133.3.1212-1223.1978.

Abstract

The fate of [3H]DNA from Streptococcus sanguis str-r43 fus-s donors in [14C]S. sanguis str-s fus-r1 recipients was studied by examining the lysates prepared from such recipients at various times after 1 min of exposure to DNA. The lysates were analyzed in CsCl and 10 to 30% sucrose gradients; fractions from the gradients were tested for biological activity and sensitivity to nucleases, subjected to various treatments and retested for nuclease sensitivity, and run on 5 to 20% neutral and alkaline sucrose gradients. The results demonstrate that donor DNA bound to S. sanguis cells in a form resistant to exogenous deoxyribonuclease is initially single stranded and complexed to recipient material. Donor DNA can be removed from the complex upon treatment of the complex with Pronase, phenol, or isoamyl alcohol-chloroform. Within the complex, donor DNA is relatively insensitive to S1 endonuclease but can regain its sensitivity by treatment with phenol. With time the complex moves as a whole to associate physically with the recipient chromosome. After a noncovalent stage of synapsis, donor material is covalently bonded to and acquires the nuclease sensitivity of recipient DNA, while donor markers regain transforming activity and become linked to resident markers.

摘要

通过检测在暴露于DNA 1分钟后的不同时间从[14C]血链球菌str-s fus-r1受体菌制备的裂解物,研究了来自血链球菌str-r43 fus-s供体菌的[3H]DNA在受体菌中的命运。裂解物在CsCl和10%至30%蔗糖梯度中进行分析;对梯度中的组分进行生物活性和核酸酶敏感性测试,进行各种处理后再测试核酸酶敏感性,并在5%至20%中性和碱性蔗糖梯度上进行分析。结果表明,以对外源脱氧核糖核酸酶有抗性的形式与血链球菌细胞结合的供体DNA最初是单链的,并与受体物质复合。用链霉蛋白酶、苯酚或异戊醇-氯仿处理复合物后,供体DNA可从复合物中去除。在复合物中,供体DNA对S1核酸内切酶相对不敏感,但用苯酚处理后可恢复其敏感性。随着时间的推移,复合物整体移动并与受体染色体发生物理结合。在非共价联会阶段之后,供体物质共价结合到受体DNA上并获得受体DNA的核酸酶敏感性,而供体标记恢复转化活性并与常驻标记相连。

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