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发菜蛋白质组双向电泳技术的建立及优化 总被引:3,自引:0,他引:3
为建立适用于发菜(Nostoc flagelliforme)蛋白质组研究的双向电泳技术,对发菜蛋白质的提取、裂解、上样量、IEF及SDS-PAGE电泳等关键步骤进行了优化,结果显示:发菜蛋白质主要分布在pH 4~7范围内,采用改良TCA法可提高提取液中蛋白质的含量和双向电泳图谱的分辨率,裂解液含60 mmol/L DTT,24 cm IPG胶条上样量1.5 mg时不仅提高了蛋白质的溶解性,而且改善了双向电泳的分离效果,得到近800个蛋白点,且蛋白点清晰,图谱分辨率较好.采用优化后的双向电泳体系提高了发菜蛋白质双向电泳的分辨率和重复性,建立起一套适用于发菜蛋白质组分析的双向电泳方法. 相似文献
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巴西橡胶树(Hevea brasiliensis)的黄色体在胶乳凝固和保护植株过程中有重要作用。本文比较使用三氯醋酸/丙酮(TCA/ ACE)、Tris缓冲液、磷酸缓冲液提取橡胶树胶乳黄色体总蛋白的双向电泳效果。确定一种适合双向电泳的蛋白提取方法。结果表明Tris缓冲液提取法得到的双向电泳图谱可以达到300个,尤其是低丰度蛋白呈现性较好,适合提取黄色体蛋白以进行双向电泳。 相似文献
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探讨适用于双向电泳的昆虫离体细胞总膜蛋白提取技术及适于双向电泳染色的高灵敏度蛋白质银染技术。以粉纹夜蛾细胞系BT1-TN-5B1-4为材料,比较了传统的Kwa法和Sigma公司的ProteoProp^TMMEMBRANE EXTRACTION KIT提取BT1-TN-5B1。离体细胞总膜蛋白,SDS—PAGE及双向电泳结果表明Sigma公司试剂盒提取的总膜蛋白效果较好,并且适用于双向电泳分析;比较了两种蛋白银染方法,确定并优化了一种灵敏度较高适于双向电泳的银染方法,得到了理想的膜蛋白2-DE图谱。 相似文献
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目的:优化双向电泳的条件,建立适用于桶形芋螺毒管蛋白质组分析的双向电泳方法。方法:对毒管蛋白的提取、上样量及SDS-PAGE凝胶浓度等影响因素进行优化。结果:乙酸提取法适宜于毒管蛋白的提取,对于pH3~10、17cm的IPG胶条,当上样量为0.75mg,聚焦70000Vhr,SDS-PAGE凝胶浓度为15%时,可提高双向电泳的分离效果,所得蛋白点清晰、数目达到1003个。结论:采用优化的条件进行双向电泳,能得到分辨率高、重现性好、完整的双向电泳图谱,为后续桶形芋螺毒管蛋白质组学研究打下基础。 相似文献
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家蚕Bombyxmori(L.)既是重要的经济昆虫,又是鳞翅目昆虫研究的典型模式生物。开展家蚕蛋白质组研究,将有助于阐明家蚕绢丝蛋白的分泌机理,也是研究鳞翅目昆虫及其他生物生命本质的需要。双向电泳是蛋白质分离的关键技术。为探讨适宜家蚕蛋白质组研究的双向电泳条件,以家蚕丝腺、丝腺内容物、蚕卵和血液为材料,在不同条件下进行双向电泳,并对分离的蛋白点进行质谱分析。结果表明:通过改进的蛋白质裂解液辅以超声破碎制备的蛋白质,双向电泳后能够得到较好的2-DE图,也能满足进行MALDI-TOFMS分析的需要。因此本研究方法适用于家蚕不同组织中蛋白质的提取和双向电泳。 相似文献
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猪卵母细胞蛋白质组双向电泳体系的建立及初步分析 总被引:1,自引:0,他引:1
建立了猪(Sus scrofa)卵母细胞蛋白质双向电泳平台,并对裂解液的组成、样品处理、双向电泳程序等相关技术进行优化,得到清晰的微量卵母细胞蛋白质的电泳图谱.利用上述优化后的体系分别对未成熟和成熟的猪卵母细胞进行双向电泳分析,并用ImageMaser软件对图谱进行比对分析.结果表明,电泳图谱上大约有800个左右的蛋白点,其中差异蛋白35个,包括上调蛋白22个及下调蛋白13个.说明基于双向电泳的蛋白质组学可以用于卵母细胞成熟的蛋白表达差异的研究. 相似文献
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建立并优化了沼泽型水牛睾丸曲精细管蛋白质分离的双向电泳体系,为后续水牛睾丸曲精细管蛋白质表达谱的鉴定和研究奠定基础。比较不同IPG胶条(线性与非线性)、胶条pH范围和蛋白质上样量这三个参数对双向电泳结果的影响。结果显示,采用上样量350μg的曲精细管总蛋白、24 cm且pH值4~7的线性IPG胶条能够更好地分离水牛睾丸曲精细管蛋白质,获得质量较好且分辨率较高的双向电泳图谱,得到大约486个蛋白点。双向凝胶电泳技术能够对水牛睾丸曲精细管蛋白质进行有效分离,并通过对双向电泳体系的优化可获得蛋白质点清晰且分辨率更高的双向电泳图谱。 相似文献
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Iu E Dubrova 《Genetika》1983,19(3):345-352
The review of literature on application of the methods of two-dimensional electrophoresis according to O'Farrel, in population genetics and in some adjacent fields of biology, is presented. Resolution capacities of both conventional and two-dimensional electrophoresis are briefly characterized. Data on application of two-dimensional electrophoresis methods for evaluation the degree of inter- and intraspecific variability, for detection and characterization of mutations, as well as for analysis of molecular mechanisms of inborn pathology are reviewed. 相似文献
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Queloz PA Crettaz D Thadikkaran L Sapin V Gallot D Jani J Deprest J Lémery D Barelli S Tissot JD 《Journal of chromatography. B, Analytical technologies in the biomedical and life sciences》2007,850(1-2):336-342
Amniotic fluid (AF) is a potential source of biomarkers for many disorders which may occur during pregnancy. The purpose of this study was to evaluate the place of two-dimensional gel electrophoresis (2-DE) technologies to compare AF in both normal and pathological situations. Two-dimensional fluorescence difference gel electrophoresis (2D-DIGE; Ettan DIGE) as well as two-dimensional gel electrophoresis and silver staining followed by image analysis were used. Differentially expressed proteins were identified by mass spectrometry. This approach was used to study electrophoregrams of normal AF obtained at 17 weeks of gestation and at term, as well as AF from fetuses presenting with congenital diaphragmatic hernia. Finally, the potential of two-dimensional electrophoresis was assessed by studying the protein profile of plasma containing AF proteins in a model of premature rupture of the membranes (PROM). Our results clearly show that two-dimensional electrophoresis technologies still have place for analyzing biological fluids such as AF. 相似文献
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Thierry Rabilloud 《Journal of Proteomics》2010,73(8):1562-1572
Electrophoretic separations of proteins are widely used in proteomic analyses, and rely heavily on SDS electrophoresis. This mode of separation is almost exclusively used when a single dimension separation is performed, and generally represents the second dimension of two-dimensional separations.Electrophoretic separations for proteomics use robust, well-established protocols. However, many variations in almost all possible parameters have been described in the literature over the years, and they may bring a decisive advantage when the limits of the classical protocols are reached.The purpose of this article is to review the most important of these variations, so that the readers can be aware of how they can improve or tune protein separations according to their needs.The chemical variations reviewed in this paper encompass gel structure, buffer systems and detergents for SDS electrophoresis, two-dimensional electrophoresis based on isoelectric focusing and two-dimensional electrophoresis based on cationic zone electrophoresis. 相似文献
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The intent of this overview is to provide the readers, especially those who are currently conducting two-dimentional electrophoresis, a basic understanding in the construction and use of microcomputer-based systems for the analysis of protein profiles generated by two-dimensional gel electrophoresis. In addition, a microcomputer-based system, employing fixed-point operations and effective algorithms, has been evaluated. The validity of this system has been demonstrated by using the two-dimensional silver-stained gels and fluorograms derived from the rat prostate. It is concluded that the present system can be used to aid the analysis of two-dimensional electrophoresis gels. An overall consideration of hardware and software components of a computer-based system is briefly discussed. 相似文献
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Genetic Variation in Proteins: Comparison of One-Dimensional and Two-Dimensional Gel Electrophoresis 总被引:2,自引:0,他引:2 
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下载免费PDF全文 Two proteins with known characteristics on one-dimensional gels were studied by two-dimensional electrophoresis to compare the sensitivities of the two methods in detecting genetic variation. Two-dimensional electrophoresis was found to be less sensitive than several types of one-dimensional gels in distinguishing variants of both proteins. Denaturation of proteins in urea in the two-dimensional method makes it possible to distinguish closely related proteins that differ from each other by units of charge. Many more types of variation in protein sequences can be distinguished on one-dimensional gels in the absence of denaturants. The estimates of heterozygosity based on two-dimensional gels are lower than those based on other methods, at least in part, because of the limited types of sequence differences that can be detected on two-dimensional gels. The application of two-dimensional electrophoresis to the measurement of genetic variation and to the detection of new mutations should be made carefully, in view of the limited sensitivity of the method in finding differences in sequence. 相似文献
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Structural proteins of active 60-S and 40-S subunits of rat liver ribosomes were analysed by two-dimensional polyacrylamide gel electrophoresis. 35 and 29 spots were shown on two-dimensional gel electrophoresis of proteins from large and small subunits, respectively. It was noted that the migration distances of stained proteins with Amido black 10B remained unchanged in the following sodium dodecyl sulfate-acrylamide gel electrophoresis, although some minor degradation and/or aggregation products were observed in the case of several ribosomal proteins, especially of those with high molecular weights. This finding made it possible to measure the molecular weight of each ribosomal protein in the spot on two-dimensional gel electrophoresis by following sodium dodecyl sulfate-acrylamide gel electrophoresis. The molecular weights of the protein components of two liver ribosomal subunits were determined by this 'three-dimensional' polyacrylamide gel electrophoresis. The molecular weights of proteins of 40-S subunits ranged from 10 000 to 38 000 and the number average molecular weight was 23 000. The molecular weights of proteins of 60-S subunits ranged from 10 000 to 60 000 and the number average molecular weight was 23 900. 相似文献
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Two-dimensional electrophoresis is an efficient method for the analysis of a broad range of complex protein samples. Current two-dimensional gel techniques are not suited for analysis of the small amount of proteins from tissue samples in the presence of high concentration of salts. Here we describe an improved two-dimensional gel electrophoresis procedure based on the use of a nonionic wetting agent, Tergitol NP7, in rehydration solution combined with the application of a linear potential sweep during isoelectrofocusing. This experimental approach yields a dramatic increase in the resolution and focusing of proteins visualized on two-dimensional gels. This technique is less time-consuming and laborious than the current techniques and can be used for a variety of two-dimensional electrophoresis applications, including proteome analysis. 相似文献
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Queloz PA Crettaz D Thadikkaran L Sapin V Tissot JD 《Protein and peptide letters》2006,13(10):959-963
To assess the efficiency of two-dimensional fluorescence difference gel electrophoresis (2D-DIGE) and of two-dimensional electrophoresis and ammoniacal silver staining (2D-E), different amounts of soybean trypsin inhibitor and horse myoglobin were added to amniotic fluid. In this model, a minimum of 5 to 10 ng of "artificial" biomarkers was detected. 相似文献
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S A Konstantinova D B Zorov L I Kovalev S S Shishkin 《Biokhimii?a (Moscow, Russia)》1991,56(11):2042-2051
Porin, a protein able to form ionic channels in model phospholipid membranes, has been isolated for the first time from bovine heart mitochondria. One-dimensional electrophoresis in the presence of sodium dodecyl sulfate revealed a major band with Mr of 32-34 kDa. On two-dimensional electrophoregrams this protein is represented by four components with pI ranging from 6.5 to 7.1. Porin spots were identified on two-dimensional electrophoregrams in a complete mixture of mitochondrial proteins. The presence of porin in bovine heart submitochondrial particles was demonstrated by two-dimensional electrophoresis. 相似文献