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解纤维醋弧菌的纤维小体系统包括一种新型衔接蛋白和一种细胞表面锚定蛋白。

The cellulosome system of Acetivibrio cellulolyticus includes a novel type of adaptor protein and a cell surface anchoring protein.

作者信息

Xu Qi, Gao Wenchen, Ding Shi-You, Kenig Rina, Shoham Yuval, Bayer Edward A, Lamed Raphael

机构信息

Department of Molecular Microbiology and Biotechnology, Tel-Aviv University, Ramat Aviv, Israel.

出版信息

J Bacteriol. 2003 Aug;185(15):4548-57. doi: 10.1128/JB.185.15.4548-4557.2003.

DOI:10.1128/JB.185.15.4548-4557.2003
PMID:12867464
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC165778/
Abstract

A scaffoldin gene cluster was identified in the mesophilic cellulolytic anaerobe Acetivibrio cellulolyticus. The previously described scaffoldin gene, cipV, encodes an N-terminal family 9 glycoside hydrolase, a family 3b cellulose-binding domain, seven cohesin domains, and a C-terminal dockerin. The gene immediately downstream of cipV was sequenced and designated scaB. The protein encoded by this gene has 942 amino acid residues and a calculated molecular weight of 100,358 and includes an N-terminal signal peptide, four type II cohesions, and a C-terminal dockerin. ScaB cohesins 1 and 2 are very closely linked. Similar, but not identical, 39-residue Thr-rich linker segments separate cohesin 2 from cohesin 3 and cohesin 3 from cohesin 4, and an 84-residue Thr-rich linker connects the fourth cohesin to a C-terminal dockerin. The scaC gene downstream of scaB codes for a 1,237-residue polypeptide that includes a signal peptide, three cohesins, and a C-terminal S-layer homology (SLH) module. A long, ca. 550-residue linker separates the third cohesin and the SLH module of ScaC and is characterized by an 18-residue Pro-Thr-Ala-Ser-rich segment that is repeated 27 times. The calculated molecular weight of the mature ScaC polypeptide (excluding the signal peptide) is 124,162. The presence of the cohesins and the conserved SLH module implies that ScaC acts as an anchoring protein. The ScaC cohesins are on a separate branch of the phylogenetic tree that is close to, but distinct from, the type I cohesins. Affinity blotting with representative recombinant probes revealed the following specific intermodular interactions: (i) an expressed CipV cohesin binds selectively to an enzyme-borne dockerin, (ii) a representative ScaB cohesin binds to the CipV band of the cell-free supernatant fraction, and (iii) a ScaC cohesin binds to the ScaB dockerin. The experimental evidence thus indicates that CipV acts as a primary (enzyme-recognizing) scaffoldin, and the protein was also designated ScaA. In addition, ScaB is thought to assume the role of an adaptor protein, which connects the primary scaffoldin (ScaA) to the cohesin-containing anchoring scaffoldin (ScaC). The cellulosome system of A. cellulolyticus thus appears to exhibit a special type of organization that reflects the function of the ScaB adaptor protein. The intercalation of three multiple cohesin-containing scaffoldins results in marked amplification of the number of enzyme subunits per cellulosome unit. At least 96 enzymes can apparently be incorporated into an individual A. cellulolyticus cellulosome. The role of such amplified enzyme incorporation and the resultant proximity of the enzymes within the cellulosome complex presumably contribute to the enhanced synergistic action and overall efficient digestion of recalcitrant forms of cellulose. Comparison of the emerging organization of the A. cellulolyticus cellulosome with the organizations in other cellulolytic bacteria revealed the diversity of the supramolecular architecture.

摘要

在嗜温性纤维素分解厌氧菌解纤维醋弧菌中鉴定出一个脚手架蛋白基因簇。先前描述的脚手架蛋白基因cipV编码一个N端9型糖苷水解酶、一个3b型纤维素结合结构域、七个粘着蛋白结构域和一个C端对接蛋白。对cipV下游紧邻的基因进行测序并命名为scaB。该基因编码的蛋白质有942个氨基酸残基,计算分子量为100358,包括一个N端信号肽、四个II型粘着蛋白和一个C端对接蛋白。ScaB的粘着蛋白1和2紧密相连。相似但不完全相同的富含苏氨酸的39个残基的连接片段将粘着蛋白2与粘着蛋白3以及粘着蛋白3与粘着蛋白4分隔开,一个84个残基的富含苏氨酸的连接子将第四个粘着蛋白与C端对接蛋白相连。scaB下游的scaC基因编码一个1237个残基的多肽,包括一个信号肽、三个粘着蛋白和一个C端S层同源(SLH)模块。一个长约550个残基的连接子将ScaC的第三个粘着蛋白和SLH模块分隔开,其特征是一个富含脯氨酸 - 苏氨酸 - 丙氨酸 - 丝氨酸的18个残基的片段重复了27次。成熟ScaC多肽(不包括信号肽)的计算分子量为124162。粘着蛋白和保守的SLH模块的存在表明ScaC作为一种锚定蛋白起作用。ScaC粘着蛋白位于系统发育树的一个单独分支上,与I型粘着蛋白接近但不同。用代表性重组探针进行的亲和印迹显示了以下特定的模块间相互作用:(i)表达的CipV粘着蛋白选择性地结合到酶携带的对接蛋白上,(ii)一个代表性的ScaB粘着蛋白结合到无细胞上清液组分的CipV条带上,(iii)一个ScaC粘着蛋白结合到ScaB对接蛋白上。因此,实验证据表明CipV作为主要的(酶识别)脚手架蛋白起作用,该蛋白也被命名为ScaA。此外,ScaB被认为承担衔接蛋白的作用,它将主要的脚手架蛋白(ScaA)与含粘着蛋白的锚定脚手架蛋白(ScaC)连接起来。因此,解纤维醋弧菌的纤维小体系统似乎呈现出一种特殊的组织类型,这反映了ScaB衔接蛋白的功能。三个含多个粘着蛋白的脚手架蛋白的插入导致每个纤维小体单元中酶亚基数量的显著增加。至少96种酶显然可以被整合到单个解纤维醋弧菌纤维小体中。这种增加的酶整合作用以及纤维小体复合物中酶的紧密相邻的作用可能有助于增强协同作用以及对顽固形式纤维素的整体高效消化。将解纤维醋弧菌纤维小体新出现的组织与其他纤维素分解细菌中的组织进行比较,揭示了超分子结构的多样性。

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