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Binding of DNA in vitro by a small, acid-soluble spore protein from Bacillus subtilis and the effect of this binding on DNA topology.

机译:枯草芽孢杆菌的一种小的酸溶性孢子蛋白在体外与DNA的结合以及这种结合对DNA拓扑结构的影响。

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摘要

The DNA within spores of Bacillus subtilis is complexed with a large amount of alpha/beta-type small, acid-soluble spore protein (SASP). Measurement of the interaction of a purified alpha/beta-type SASP with DNA in vitro by a filter binding assay showed that the binding saturated at one molecule of SASP per approximately 5 bp. SASP-DNA binding did not require a divalent cation, was optimal at pH 6.7, and was unaffected by salt up to 400 mM. Binding of SASP to relaxed plasmid DNA in the presence of topoisomerase I resulted in the introduction of 18 (for plasmid pUC19) or 36 (for plasmid pUB110) negative supertwists, a superhelical density similar to that found in several plasmids isolated from spores. The SASP-dependent introduction of negative supertwists did not require a divalent cation, was unaffected by salt, and also gave a value of one molecule of SASP per approximately 5 bp at saturation. There was at least one slow step in the binding of SASP to DNA as seen in both the filter binding and supercoiling assays.
机译:枯草芽孢杆菌孢子内的DNA与大量的α/β型小酸溶性孢子蛋白(SASP)形成复合物。通过过滤器结合测定法测量纯化的α/β型SASP与DNA的体外相互作用,结果表明结合大约每5 bp在一个SASP分子处达到饱和。 SASP-DNA结合不需要二价阳离子,在pH 6.7最佳,并且不受高达400 mM盐的影响。在拓扑异构酶I存在下SASP与松弛质粒DNA的结合导致引入18个(对于质粒pUC19)或36个(对于质粒pUB110)负超捻,其超螺旋密度类似于在从孢子中分离的几种质粒中发现的超螺旋密度。依赖于SASP的阴性超捻分子的引入不需要二价阳离子,不受盐的影响,并且饱和时每5 bp产生一个SASP分子值。如在滤纸结合和超螺旋测定中所见,SASP与DNA的结合至少有一个缓慢的步骤。

著录项

  • 作者单位
  • 年度 1990
  • 总页数
  • 原文格式 PDF
  • 正文语种 en
  • 中图分类
  • 入库时间 2022-08-20 20:39:25

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