Ⅳ型限制酶ScoMcrA中SRA结构域介导的二聚体化对硫结合结构域功能的影响机制

【背景】部分细菌的DNA骨架会发生磷硫酰化修饰,硫结合结构域(Sulfur Binding Domain,SBD)可以特异性识别这种生理修饰。与绝大多数SBD-HNH双结构域核酸酶不同,ScoMcrA的SBD和HNH结构域中间插入了一个特异性识别5-甲基胞嘧啶(5m C)修饰DNA的SET and RING-Associated(SRA)结构域。晶体结构显示,单独的SBD是单体,而SBD-SRA是双体。【目的】探究ScoMcrA中SRA结构域的存在对SBD识别硫修饰DNA的影响及影响方式。【方法】凝胶迁移实验(Electrophoresis Mobility Shift Assay,EMSA)比较SBD、SBD-SRA对硫修饰DNA结合力的差异;对参与SBD-SRA二聚体化的关键氨基酸残基突变,并检测点突变对SBD-SRA蛋白二聚体化及结合硫修饰DNA的影响。【结果】相较于SBD结构域,SBD-SRA双结构域对磷硫酰化修饰DNA的结合能力明显增强。对SBD-SRA双体互作界面进行单点突变基本不影响其对硫修饰DNA的结合,当二聚体化界面连续的L261LGET265突变成A261AAAA265时,突变体对硫修饰DNA的结合力下降到与SBD相似的水平。【结论】根据EMSA实验结果可以初步判断,SRA结构域介导的SBD-SRA双体化能增强SBD对硫修饰DNA的结合力;L261LGET265是SRA结构域上影响SBD对硫修饰DNA结合力的关键氨基酸位点。     

灭癌素链霉菌中磷硫酰化修饰DNA结合结构域的功能分析

[目的]DNA磷硫酰化(phosphorothioation,PT)是由硫原子取代DNA骨架磷原子上的非桥联氧原子形成的一种新型DNA修饰.PT修饰除参与组成限制修饰系统外,其更为广泛的生物学功能仍有待揭示.PT修饰现有的检测方法操作复杂、成本高、耗时长,而具有操作简便、成本低、耗时短等特点的酶联免疫检测(enzyme...     

B结构域糖基化位点对凝血因子Ⅷ分泌和活性的影响

目的:研究B结构域糖基化位点对凝血因子Ⅷ分泌和活性的影响。方法:通过反向PCR技术在凝血因子ⅧA2和A3结构域之间插入B结构域的糖基化序列,PCR后进行重组连接、质粒转化、克隆筛选、质粒抽提等步骤,构建重组人凝血因子Ⅷ载体,然后再通过活性检测试剂盒检测胞外分泌因子Ⅷ活性,用ELISA(双抗体夹心法)检测胞外分泌因子Ⅷ总表达,用Western印迹检测重组因子Ⅷ在胞内的总表达。结果:B结构域糖基化点的增加使得因子Ⅷ的胞外相对活性最高提高了1倍。结论:糖基化位点的加入可以增强因子Ⅷ的胞外活性,如果适当增加糖基化位点的长度和数量(单个糖基化位点重复出现或多个糖基化位点连接),可以进一步提高因子Ⅷ的胞外表达和活性。     

一氧化氮合酶FMN结合结构域的电子传递及调控机制研究现状

生物体内NO是在一氧化氮合酶（mitric oxide synthase,NOS）催化下生成的,NOS的结构包括C端还原酶域和N端加氧酶域。还原酶域中的FMN结合结构域既可接受来自NADPH-FAD结构域的电子,又可作为提供电子的供体,在调控催化过程中的电子传递方面发挥着重要作用。主要从FMN结合结构域的构象平衡及其对不同亚型NOS的动力学差异的贡献、FMN结合结构域自身的电荷性质以及NOS中其他结构域对FMN结构域的功能调控三个方面进行了论述,以期揭示NOS独特的电子传递催化机制。     

内毒素耐受对核苷酸结合寡聚化结构域2信号通路的影响

为研究内毒素耐受对核苷酸结合寡聚化结构域2(nucleotide-binding oligomerization domain containing 2,NOD2)信号通路的影响,将小鼠单核-巨噬细胞RAW264.7分为两组,分别给予小剂量脂多糖(lipopolysaccharide,LPS)(100ng/mL)或磷酸盐缓冲液(phosphate buffered saline,PBS)预处理20h,建立内毒素耐受组和对照组。每组细胞分别给予大剂量LPS(1 000ng/mL)或热灭活烟曲霉孢子刺激,于刺激后0、2、6、12、24h采用定量聚合酶链反应(polymerase chain reaction,PCR)检测细胞NOD2、受体相互作用蛋白2(receptor-interacting protein 2,RIP2)和肿瘤坏死因子α(tumor necrosis factorα,TNF-α)mRNA表达;采用酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)检测细胞上清液中白细胞介素8(interleukin 8,IL-8)和TNF-α浓度。结果显示,内毒素耐受组无论是大剂量LPS还是热灭活烟曲霉孢子刺激均不能增加NOD2、RIP2和TNF-αmRNA表达及细胞上清液中IL-8、TNF-α浓度;而对照组大剂量LPS和热灭活烟曲霉孢子刺激均可提高NOD2、RIP2和TNF-αmRNA表达及细胞上清液中IL-8、TNF-α浓度,尤以刺激后12h增加显著,与刺激前(0h)比较,差异有统计学意义(P0.05)。结果提示,内毒素耐受可能对NOD2信号通路有抑制作用。     

Salmonella enteric硫修饰蛋白DptC半胱氨酸定点突变对Dnd表型的影响

[目的]Salmonella enterica serovar Cerro 87是具有硫修饰现象即Dnd表型的细菌之一,其硫修饰受dptBCDE基因簇控制,将dptBCDE克隆、转化Escherichia coli DH10B后,可赋予后者Dnd表型,而当其中dptC缺失后,Dnd表型随之丧失.本文探索S.enterica serovar Cerro 87硫修饰基因dptC在硫修饰发生过程中的作用.[方法]将DptC中6个半胱氨酸(Cys)在DNA水平上逐个定点突变,转化携带dptBCDE及其衍生系列的质粒至E.coli DH10B,检测相应受体菌Dnd表型.[结果]在DptC的6个Cys中,除C39外,其余5个突变均可导致Dnd表型丧失,说明DptC中C146、C262、C273、C280和C283均与硫修饰有关.生物信息学分析表明,这5个Cys在硫修饰细菌科属间高度保守,佐证了S.enteric DptC中这5个Cys与硫修饰有关的结论.[结论]S.enteric DptC中C146、C262、C273、C280和C283任何一个的突变,都会导致受体菌Dnd表型丧失.该结果为进一步探索DNA硫修饰的发生机制提供了线索.     

安丝菌素聚酮合酶模块2中脱水酶结构域的生化功能

[目的]I型聚酮合酶(Polyketide synthase,PKS)模块中不同的修饰是聚酮类化合物结构多样性的重要原因之一.抗癌药物安丝菌素化学结构中C11-C14区域存在特殊的双键迁移结构,可能与聚酮合酶模块2或者3中脱水酶结构域(Dehydratase,DH)的催化密切相关,本研究通过探究聚酮合酶模块2中DH结构...     

水稻OsGAP1 C2结构域中对钙离子的结合能力强于对钾离子

钙离子作为植物细胞的第二信使,广泛参与植物应对不同逆境胁迫的信号调控过程。水稻G蛋白促进蛋白1（Oryza sativa GTPase activating protein 1, OsGAP1）包含1个C2结构域,而含C2结构域的蛋白质是一类钙离子结合蛋白质,受钙信号的调控。本研究鉴定了水稻OsGAP1的由5个保守性天冬氨酸残基组成的阳离子结合区域。该区域可结合2个钙离子或者钾离子,且其结合钙离子的强度高于其结合钾离子的强度,但是不能结合镁离子。当将其中2个保守的天冬氨酸残基(Asp-23和Asp-28)突变为丙氨酸后,其对钙离子的结合能力减弱。对OsGAP1 C2结构域阳离子结合区域结合金属离子能力的研究,有助于加深对钙信号调控蛋白质的认识,为其在农业生产中的应用提供理论依据。     

水稻OsGAP1 C2结构域中对钙离子的结合能力强于对钾离子北大核心CSCD

钙离子作为植物细胞的第二信使,广泛参与植物应对不同逆境胁迫的信号调控过程。水稻G蛋白促进蛋白1(Oryza sativa GTPase-activating protein 1,OsGAP1)包含1个C2结构域,而含C2结构域的蛋白质是一类钙离子结合蛋白质,受钙信号的调控。本研究鉴定了水稻OsGAP1的由5个保守性天冬氨酸残基组成的阳离子结合区域。该区域可结合2个钙离子或者钾离子,且其结合钙离子的强度高于其结合钾离子的强度,但是不能结合镁离子。当将其中2个保守的天冬氨酸残基(Asp-23和Asp-28)突变为丙氨酸后,其对钙离子的结合能力减弱。对OsGAP1 C2结构域阳离子结合区域结合金属离子能力的研究,有助于加深对钙信号调控蛋白质的认识,为其在农业生产中的应用提供理论依据。     

血清硫氧还蛋白相互作用蛋白、Ⅲ型纤维蛋白结构域结合蛋白5与糖尿病性心肌病的相关性及诊断价值分析

摘要 目的：分析血清硫氧还蛋白相互作用蛋白（TXNIP）、Ⅲ型纤维蛋白结构域结合蛋白5（FNDC5）与糖尿病性心肌病的相关性及诊断价值。方法：选择我院自2019年10月至2022年10月接诊的128例糖尿病患者作为研究对象,其中糖尿病性心肌病53例,作为观察组;左心室二维结构正常75例,作为对照组。检测两组血清TXNIP、FNDC5表达水平,分析糖尿病性心肌病患者血清TXNIP、FNDC5表达水平与左心功能指标的关系,使用多因素Logistic回归分析及ROC曲线分析血清TXNIP、FNDC5对糖尿病性心肌病的诊断价值。结果：观察组血清TXNIP表达水平高于对照组,FNDC5表达水平低于对照组,差异均有统计学意义（P＜0.05）;经Pearson相关性分析,糖尿病性心肌病患者二尖瓣早期血流速度峰值(E)、左侧壁二尖瓣环早期峰值速度均值（e''）、左心室射血分数（LVEF）均与TXNIP呈负相关,与FNDC5呈正相关（P＜0.05）;经多因素Logistic回归分析,血清TXNIP、FNDC5均是糖尿病性心肌病的独立预测因素（P＜0.05）;经ROC曲线分析,血清TXNIP联合FNDC5诊断糖尿病性心肌病的AUC为0.926,明显大于单一指标TXNIP的0.671和FNDC5的0.685,差异均有统计学意义（P＜0.05）。结论：血清TXNIP、FNDC5与糖尿病性心肌病发病及患者左心功能损害程度密切相关,两者联合诊断此病的效能较好,值得临床进一步研究应用。     

Cleavage of phosphorothioated DNA and methylated DNA by the type IV restriction endonuclease ScoMcrA

Many taxonomically diverse prokaryotes enzymatically modify their DNA by replacing a non-bridging oxygen with a sulfur atom at specific sequences. The biological implications of this DNA S-modification (phosphorothioation) were unknown. We observed that simultaneous expression of the dndA-E gene cluster from Streptomyces lividans 66, which is responsible for the DNA S-modification, and the putative Streptomyces coelicolor A(3)2 Type IV methyl-dependent restriction endonuclease ScoA3McrA (Sco4631) leads to cell death in the same host. A His-tagged derivative of ScoA3McrA cleaved S-modified DNA and also Dcm-methylated DNA in vitro near the respective modification sites. Double-strand cleavage occurred 16-28 nucleotides away from the phosphorothioate links. DNase I footprinting demonstrated binding of ScoA3McrA to the Dcm methylation site, but no clear binding could be detected at the S-modified site under cleavage conditions. This is the first report of in vitro endonuclease activity of a McrA homologue and also the first demonstration of an enzyme that specifically cleaves S-modified DNA.     

Site directed mutagenesis of Histidine residues in Anthrax toxin lethal factor binding domain reduces toxicity

Anthrax lethal toxin is a mixture of protective antigen (PA, 735 AA) and lethal factor (LF, 776 AA). Earlier studies have shown that 254 residues of lethal factor are sufficient for PA binding to cause internalization (Arora N and Leppla SH, J Biol Chem 268: 3334-3342, 1993). The present study was undertaken to determine residues which are important for binding of LF to PA. LF modification with diethyl pyrocarbonate (DEPC, modifies histidine residue primarily) results in the loss of binding and toxicity in mammalian cells. There are nine histidine residues in the binding domain. To locate the important residue(s), site-directed mutagenesis of these histidines were performed by recombinant methods. Replacement of His42 with Gly42 destablizes the protein and hence it could not be purified. His35 when mutagenized to Gly35 (mLF-DTA) diminishes the toxicity by 20 fold. Time dependent studies show that binding of mLF-DTA was reduced at shorter incubations and longer incubations taper off this difference. Gel shift assay suggested 8-10% less binding of mLF-DTA as compared to LF-DTA. In conclusion His35 is important for binding and His42 is critical and confers proper conformation for LF binding to PA.     

Probing the ligand binding domain of the GluR2 receptor by proteolysis and deletion mutagenesis defines domain boundaries and yields a crystallizable construct.

Ionotropic glutamate receptors constitute an important family of ligand-gated ion channels for which there is little biochemical or structural data. Here we probe the domain structure and boundaries of the ligand binding domain of the AMPA-sensitive GluR2 receptor by limited proteolysis and deletion mutagenesis. To identify the proteolytic fragments, Maldi mass spectrometry and N-terminal amino acid sequencing were employed. Trypsin digestion of HS1S2 (Chen GQ, Gouaux E. 1997. Proc Natl Acad Sci USA 94:13431-13436) in the presence and absence of glutamate showed that the ligand stabilized the S1 and S2 fragments against complete digestion. Using limited proteolysis and multiple sequence alignments of glutamate receptors as guides, nine constructs were made, folded, and screened for ligand binding activity. From this screen, the S1S21 construct proved to be trypsin- and chymotrypsin-resistant, stable to storage at 4 degrees C, and amenable to three-dimensional crystal formation. The HS1S21 variant was readily prepared on a large scale, the His tag was easily removed by trypsin, and crystals were produced that diffracted to beyond 1.5 A resolution. These experiments, for the first time, pave the way to economical overproduction of the ligand binding domains of glutamate receptors and more accurately map the boundaries of the ligand binding domain.     

Improving the binding affinity of an antibody using molecular modeling and site-directed mutagenesis

Activated Factor X releases F1.2, a 271-amino acid peptide, from the amino terminus of prothrombin during blood coagulation. A nine-amino acid peptide, C9 (DSDRAIEGR), corresponding to the carboxyl terminus of F1.2 was synthesized and used to produce a monoclonal antibody, TA1 (K(D)) 1.22 x 10(-6) M). To model the TA1 antibody, we entered the sequence information of the cloned TA1 Fv into the antibody modeling program, ABM, which combines homology methods, conformational search procedures, and energy screening and has proved to be a reliable and reproducible antibody modeling method. Using a novel protein fusion procedure, we expressed the C9 peptide fused to the carboxyl terminus of the PENI repressor protein from Bacillus licheniformis in Escherichia coli. We constructed fusion proteins containing alanine substitutions for each amino acid in the C9 epitope. Binding studies, using the C9 alanine mutants and TA1, and spatial constraints predicted by the modeled TA1 binding cleft enabled us to establish a plausible conformation for C9 complexed with TA1. Furthermore, based on binding results of conservative amino acid substitutions in C9 and mutations in the antibody, we were able to refine the complex model and identify antibody mutations that would improve binding affinity.     

鉴别杰多霉素生物合成后修饰氧化酶JadH中参与底物结合或催化的关键残基

JadH是羟化脱水双功能酶,参与杰多霉素生物合成中的聚酮后修饰反应,将2,3-dehydro-UWM6催化为dehydrorabelomycin。为了分析杰多霉素生物合成途径中后修饰氧化酶JadH结合、催化底物的关键氨基酸,构建了JadH与底物复合物的三维结构模型。利用该模型并结合JadH同源蛋白氨基酸序列比对分析,推测出JadH活性中心中可能参与底物结合或催化的关键氨基酸(R50、G51、L52、G53、F100、R221、I223、P295和G298)。通过定点突变及体外酶学实验对这些位点的突变体的催化活性进行评价,结果显示这些突变株活性均显著低于野生型,表明这9个氨基酸是JadH参与底物结合或催化的关键氨基酸。     

Mutations that modify or exclude binding of the QA ubiquinone and carotenoid in the reaction center from Rhodobacter sphaeroides

Three single-site mutations have been introduced at positions close to the Q_A ubiquinone in the reaction centre from Rhodobacter sphaeroides. Two of these mutations, Ala M260 to Trp and Ala M248 to Trp, result in a reaction centre that does not support photosynthetic growth of the bacterium, and in which electron transfer to the Q_A ubiquinone is abolished. In the reaction centre with an Ala to Trp mutation at the M260 residue, electron transfer from the primary donor to the acceptor bacteriopheophytin is not affected by the mutation, but electron transfer from the acceptor bacteriopheophytin to Q_A is not observed. The most likely basis for these effects is that the mutation produces a structural change that excludes binding of the Q_A ubiquinone. A third mutation, Leu M215 to Trp, produces a reaction centre that has an impaired capacity for supporting photosynthetic growth. The mutation changes the nature of ubiquinone binding at the Q_A site, and renders the site sensitive to quinone site inhibitors such as o- phenanthroline. Adopting a similar approach, in which a small residue located close to a cofactor is changed to a more bulky residue, we show that the reaction centre can be rendered carotenoid-less by the mutation Gly M71 to Leu.     

Structure-function relationship in the globular type III antifreeze protein: identification of a cluster of surface residues required for binding to ice.

Antifreeze proteins (AFPs) depress the freezing point of aqueous solutions by binding to and inhibiting the growth of ice. Whereas the ice-binding surface of some fish AFPs is suggested by their linear, repetitive, hydrogen bonding motifs, the 66-amino-acid-long Type III AFP has a compact, globular fold without any obvious periodicity. In the structure, 9 beta-strands are paired to form 2 triple-stranded antiparallel sheets and 1 double-stranded antiparallel sheet, with the 2 triple sheets arranged as an orthogonal beta-sandwich (Sönnichsen FD, Sykes BD, Chao H, Davies PL, 1993, Science 259:1154-1157). Based on its structure and an alignment of Type III AFP isoform sequences, a cluster of conserved, polar, surface-accessible amino acids (N14, T18, Q44, and N46) was noted on and around the triple-stranded sheet near the C-terminus. At 3 of these sites, mutations that switched amide and hydroxyl groups caused a large decrease in antifreeze activity, but amide to carboxylic acid changes produced AFPs that were fully active at pH 3 and pH 6. This is consistent with the observation that Type III AFP is optimally active from pH 2 to pH 11. At a concentration of 1 mg/mL, Q44T, N14S, and T18N had 50%, 25%, and 10% of the activity of wild-type antifreeze, respectively. The effects of the mutations were cumulative, such that the double mutant N14S/Q44T had 10% of the wild-type activity and the triple mutant N14S/T18N/Q44T had no activity. All mutants with reduced activity were shown to be correctly folded by NMR spectroscopy. Moreover, a complete characterization of the triple mutant by 2-dimensional NMR spectroscopy indicated that the individual and combined mutations did not significantly alter the structure of these proteins. These results suggest that the C-terminal beta-sheet of Type III AFP is primarily responsible for antifreeze activity, and they identify N14, T18, and Q44 as key residues for the AFP-ice interaction.     

Assignment of the nucleotide binding sites and the mechanism of substrate inhibition of Escherichia coli adenylate kinase

Site-directed mutagenesis of key amino acids of adenylate kinase has been used to suggest a new model for the location of the AMP and ATP binding sites. Phe-86 and Tyr-133, which are in close contact with the inhibitor Ap5A according to previous crystallographic results, have been independently changed to tryptophan and other amino acids. The Phe-86----Trp mutant had a 3- to 6-fold change in the Km for ATP and a 44-fold increase in the Km for AMP with a simultaneous loss of AMP substrate inhibition. Thus Phe-86 is probably in close contact with bound AMP. The Tyr-133----Trp mutant showed no large effects on enzyme kinetics and suggests that the previous assignment of Ap5A occupying natural adenosine binding sites is probably incorrect. A temperature-sensitive Leu-107----Gln mutant showed a 6-fold decrease in the Km for ATP and no effect on AMP binding, suggesting that this amino acid is near the ATP binding site. Changes in the fluorescence of single tryptophan-containing mutant enzymes provided specific information about AMP and ATP binding. The fluorescence results are consistent with the kinetic studies, and also suggest that AMP substrate inhibition is caused by the formation of an abortive complex that prevents the release of product.