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大肠杆菌单链结合蛋白DNA结合协同性的盐依赖性变化

Salt-dependent changes in the DNA binding co-operativity of Escherichia coli single strand binding protein.

作者信息

Lohman T M, Overman L B, Datta S

出版信息

J Mol Biol. 1986 Feb 20;187(4):603-15. doi: 10.1016/0022-2836(86)90338-4.

Abstract

The co-operative nature of the binding of the Escherichia coli single strand binding protein (SSB) to single-stranded nucleic acids has been examined over a range of salt concentrations (NaCl and MgCl2) to determine if different degrees of binding co-operativity are associated with the two SSB binding modes that have been identified recently. Quantitative estimates of the binding properties, including the co-operativity parameter, omega, of SSB to single-stranded DNA and RNA homopolynucleotides have been obtained from equilibrium binding isotherms, at high salt (greater than or equal to 0.2 M-NaCl), by monitoring the fluorescence quenching of the SSB upon binding. Under these high salt conditions, where only the high site size SSB binding mode exists (65 +/- 5 nucleotides per tetramer), we find only moderate co-operativity for SSB binding to both DNA and RNA, (omega = 50 +/- 10), independent of the concentration of salt. This value for omega is much lower than most previous estimates. At lower concentrations of NaCl, where the low site size SSB binding mode (33 +/- 3 nucleotides/tetramer) exists, but where SSB affinity for single-stranded DNA is too high to estimate co-operativity from classical binding isotherms, we have used an agarose gel electrophoresis technique to qualitatively examine SSB co-operativity with single-stranded (ss) M13 phage DNA. The apparent binding co-operativity increases dramatically below 0.20 M-NaCl, as judged by the extremely non-random distribution of SSB among the ssM13 DNA population at low SSB to DNA ratios. However, the highly co-operative complexes are not at equilibrium at low SSB/DNA binding densities, but are formed only transiently when SSB and ssDNA are directly mixed at low concentrations of NaCl. The conversions of these metastable, highly co-operative SSB-ssDNA complexes to their equilibrium, low co-operativity form is very slow at low concentrations of NaCl. At equilibrium, the SSB-ssDNA complexes seem to possess the same low degree of co-operativity (omega = 50 +/- 10) under all conditions tested. However, the highly co-operative mode of SSB binding, although metastable, may be important during non-equilibrium processes such as DNA replication. The possible relation between the two SSB binding modes, which differ in site size by a factor of two, and the high and low co-operativity complexes, which we report here, is discussed.

摘要

在一系列盐浓度(氯化钠和氯化镁)范围内,研究了大肠杆菌单链结合蛋白(SSB)与单链核酸结合的协同性质,以确定不同程度的结合协同性是否与最近确定的两种SSB结合模式相关。通过监测结合时SSB的荧光猝灭,从高盐(大于或等于0.2M氯化钠)下的平衡结合等温线获得了SSB与单链DNA和RNA同聚核苷酸结合性质的定量估计,包括协同参数ω。在这些仅存在高位点大小SSB结合模式(每个四聚体65±5个核苷酸)的高盐条件下,我们发现SSB与DNA和RNA结合时的协同性都适中(ω = 50±10),与盐浓度无关。这个ω值远低于大多数先前的估计。在较低浓度的氯化钠下,存在低位点大小SSB结合模式(33±3个核苷酸/四聚体),但SSB对单链DNA的亲和力过高,无法从经典结合等温线估计协同性,我们使用琼脂糖凝胶电泳技术定性地研究了SSB与单链(ss)M13噬菌体DNA的协同性。在低SSB与DNA比例下,通过ssM13 DNA群体中SSB的极非随机分布判断,表观结合协同性在低于0.20M氯化钠时急剧增加。然而,在低SSB/DNA结合密度下,高度协同的复合物并不处于平衡状态,而是仅在低浓度氯化钠下直接混合SSB和ssDNA时短暂形成。在低浓度氯化钠下,这些亚稳态、高度协同的SSB-ssDNA复合物向其平衡、低协同性形式的转变非常缓慢。在平衡状态下,在所有测试条件下,SSB-ssDNA复合物似乎都具有相同的低协同性程度(ω = 50±10)。然而,SSB结合的高度协同模式虽然是亚稳态的,但在DNA复制等非平衡过程中可能很重要。本文讨论了两种位点大小相差两倍的SSB结合模式与我们在此报道的高协同性和低协同性复合物之间的可能关系。

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