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连接体在蚯蚓3.6兆道尔顿六边形双层血红蛋白重新组装中的作用。

The role of linkers in the reassembly of the 3.6 MDa hexagonal bilayer hemoglobin from Lumbricus terrestris.

作者信息

Kuchumov A R, Taveau J C, Lamy J N, Wall J S, Weber R E, Vinogradov S N

机构信息

Department of Biochemistry and Molecular Biology, School of Medicine, Wayne State University, Detroit, MI, 48201, USA.

出版信息

J Mol Biol. 1999 Jun 25;289(5):1361-74. doi: 10.1006/jmbi.1999.2825.

Abstract

The extent and kinetics of reassembly of the four groups of linkers L1-L4 with 213 kDa subassemblies of twelve globin chains D, (bac)3(d)3, isolated from the approximately 3.6 MDa hexagonal bilayer (HBL) hemoglobin (Hb) of Lumbricus terrestris, was investigated using gel filtration. The reassembled HBL's were characterized by scanning transmission electron microscopic (STEM) mass mapping and their subunit content determined by reversed-phase chromatography. In reassembly by method (A), the linkers isolated by RP-HPLC at pH approximately 2.2 were added to D at neutral pH; in method (B), the linkers were renatured at neutral pH and then added to D. With method (A) the percentage of HBL reassembly varied from >/=13% in the absence of Ca(II) to </=75% in 1-10 mM Ca(II). Reassembly to HBL structures whose linker contents, STEM images and masses were similar to the native Hb was observed with all the linkers (>/=75%), with ternary and binary linker combinations (40-50%) and with individual linkers producing yields increasing in the following order: L1=1-3%, L2 approximately L3=10-20% and L4=35-55%. The yield was two- to eightfold lower with method (B), except in the case of linkers L1-L3. Although the reassembly kinetics were always biphasic, with t1/2=0.3-3.3 hours and 10-480 hours, the ratio of the amplitudes fast:slow was 1:0.6 with method (A) and 1:2.5 with method (B). These results are consistent with a scheme in which the slow HBL reassembly is dependent on a slow conversion of linker conformation at neutral pH from a reassembly incompetent to a reassembly competent conformation. Although all the linkers self-associate extensively at neutral pH, forming complexes ranging from dimers to >18-mers, the size of the complex does not affect the extent or rate of reassembly. The oxygen binding affinity of reassembled HBLs was similar to that of the native Hb, but their cooperativity was lower. A model of HBL reassembly was proposed which postulates that binding of linker dimers to two of the three T subunits of D causes conformational alterations resulting in the formation of complementary binding sites which permit lateral self-association of D subassemblies, and thus dictate the formation of a hexagonal structure due to the 3-fold symmetry of D.

摘要

使用凝胶过滤法研究了四组连接体L1 - L4与从地龙约3.6 MDa六方双层(HBL)血红蛋白(Hb)中分离出的十二条珠蛋白链D的213 kDa亚组装体重新组装的程度和动力学。通过扫描透射电子显微镜(STEM)质量映射对重新组装的HBL进行表征,并通过反相色谱法测定其亚基含量。在方法(A)的重新组装中,通过RP - HPLC在pH约2.2下分离的连接体在中性pH下添加到D中;在方法(B)中,连接体在中性pH下复性,然后添加到D中。采用方法(A)时,HBL重新组装的百分比在不存在Ca(II)时大于等于13%,在1 - 10 mM Ca(II)时小于等于75%。观察到所有连接体(大于等于75%)、三元和二元连接体组合(40 - 50%)以及单个连接体重新组装成连接体含量、STEM图像和质量与天然Hb相似的HBL结构,且单个连接体产生的产率按以下顺序增加:L1 = 1 - 3%,L2约等于L3 = 10 - 20%,L4 = 35 - 55%。除了连接体L1 - L3的情况外,方法(B)的产率低两到八倍。尽管重新组装动力学始终是双相的,t1/2 = 0.3 - 3.3小时和10 - 480小时,但快速:慢速的幅度比在方法(A)中为1:0.6,在方法(B)中为1:2.5。这些结果与一种方案一致,即缓慢的HBL重新组装依赖于连接体构象在中性pH下从无重新组装能力的构象缓慢转变为有重新组装能力的构象。尽管所有连接体在中性pH下广泛自缔合,形成从二聚体到大于18聚体的复合物,但复合物的大小并不影响重新组装的程度或速率。重新组装的HBL的氧结合亲和力与天然Hb相似,但其协同性较低。提出了一个HBL重新组装模型,该模型假设连接体二聚体与D的三个T亚基中的两个结合会导致构象改变,从而形成互补结合位点,允许D亚组装体横向自缔合,因此由于D的三重对称性决定了六边形结构的形成。

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