植物细胞壁蛋白质组学研究进展

植物细胞壁蛋白质在细胞代谢和发育调控、细胞壁组分修饰、信号转导及胁迫响应等生物学事件中具有重要功能.最近,国内外学者开展了大量植物细胞壁蛋白质组学的研究工作,并取得了巨大进展.本文详述了细胞壁蛋白质的分类、提取、鉴定及生物信息学分析的最新进展,总结了植物细胞壁蛋白质组学的应用和面临的挑战,提出了植物细胞壁蛋白质组学研究的框架图,以期为植物细胞壁蛋白质组学的广泛研究提供借鉴.     

叶绿体蛋白质组研究进展

亚细胞蛋白质组学是近年来蛋白组学研究中的一个热点。通过细胞器的纯化和亚细胞组分的分离,降低了样品的复杂性,增大了相应蛋白质组分的富集,有利于由此分离获得的蛋白质的序列分析及功能鉴定。叶绿体蛋白质组为植物亚细胞蛋白质组学研究中相对全面的一部分,利用亚细胞分离结合双向电泳技术系统地鉴定叶绿体中蛋白质组分是获取叶绿体蛋白质信息、确定其功能的重要技术手段。本文就近年来植物叶绿体蛋白质组涵盖的叶绿体内、外被膜、叶绿体基质、类囊体膜和类囊体腔蛋白的研究进行综述,以全面认识叶绿体蛋白的组成、特点及其在叶绿体生理生化代谢网络中的作用。     

脂蛋白质组学研究进展

脂蛋白质组学(lipoproteomics)是一门应用蛋白质组学技术对脂蛋白(lipoprotein)进行全面、系统地分析和鉴定,进而了解脂蛋白的组成和功能以及与相关疾病发生、发展之间关系的新兴学科.近些年来,脂蛋白质组学研究促进了脂蛋白中蛋白质组分的急性期响应、补体激活、免疫响应、炎症响应、蛋白酶抑制等新功能的发现,显示了广阔的应用前景.本文对脂蛋白的功能和分类,以及目前应用于脂蛋白质组学研究的脂蛋白分离方法和蛋白质鉴定方法进行了简述,并综述了高密度脂蛋白、低密度脂蛋白和极低密度脂蛋白的脂蛋白质组学研究,及其在冠状动脉疾病、糖尿病、类风湿性关节炎等疾病研究的最新进展.     

质谱鉴定PC12细胞蛋白酶体抑制剂PSI-诱导性包含体中的LBs蛋白质

路易(小)体(Lewy body, LB）构成特征的蛋白质组份（protein content）在体外形成的路易(小)体样包含体（Lewy body-like inclusion）或聚集体（aggresome）中能够获得鉴定．通过蛋白质组学方法鉴定LB蛋白质组分是一种新的途径.10 µmol/L人工合成蛋白酶体抑制剂PSI（proteasomal inhibitor）作用PC12细胞48 h使其产生PSI诱导性包含体（PSI-induced inclusions）. 为了在体外指明可能的LB蛋白质组分,通过生物化学分级分离、双向电泳（two-dimensional electrophoresis,2-D）和肽质量指纹鉴定（identification via peptide mass fingerprints,PMF）的蛋白质组学方法,鉴定了2个涉及突触递质合成的蛋白质、6个26 S蛋白酶体亚基、2个细胞骨架蛋白、2个线粒体蛋白、1个抗氧化蛋白和7个分子伴侣蛋白和（或）分子伴侣样蛋白等20个LB蛋白质组分.结果提示,当PC12细胞发生蛋白酶体抑制时,这20个LB蛋白质组分可能被富集到PSI诱导性包含体中．     

土壤宏蛋白质组学在土壤污染评价中的应用

土壤微生物指标是评价土壤污染程度的重要生物学指标之一.近年来,随着分子生物学的发展,应用宏基因组学、宏转录组学和宏蛋白质组学技术考察土壤微生物的生态功能成为土壤功能的研究热点.相对于宏基因组学和宏转录组学,土壤宏蛋白质组学是以土壤微生物基因的功能组分——蛋白质为直接研究对象,考察不同时空点提取出来的土壤蛋白质的变化规律,更有助于揭示土壤微生物的生态功能及其在污染物迁移转化过程中的作用,在评价土壤污染方面也更具潜力.目前,土壤宏蛋白质组学正处于起步阶段,而土壤蛋白质的提取方法是制约其发展的主要因素之一,因此本文综述了蛋白质作为土壤污染评价指标的优势,重点比较了不同土壤蛋白质提取方法的优劣,结合案例分析了蛋白质作为土壤污染评价指标的可行性及存在的问题,并对土壤宏蛋白质组学的发展进行展望.     

叶绿体蛋白质组学研究进展

蛋白质组分析是鉴定蛋白质种类和功能的有力工具之一。叶绿体作为光合作用的重要细胞器,叶绿体蛋白质组学成为了研究的热点,涉及的领域包括叶绿体的总蛋白质组学、亚细胞蛋白质组学、差异蛋白质组学和蛋白质的功能等。现主要介绍蛋白质组学的常用技术以及叶绿体蛋白质组学的最新研究进展。     

亚细胞蛋白质组研究进展

运用蛋白质组学方法对亚细胞组分进行研究是目前的研究热点。传统的亚细胞分离技术结合质谱鉴定技术为亚细胞蛋白质组学的研究提供了技术平台。本文对快速发展的亚细胞蛋白质组研究进展及其所揭示的生物学意义进行了综述。     

蛋白质组学技术及其在心血管疾病研究中的应用

蛋白质组学是旨在研究蛋白质表达谱和蛋白质与蛋白质之间相互作用的新的领域。蛋白质组学的研究必须依赖高通量、自动化程度很高的技术。双向电泳、液相色谱和生物质谱技术的发展推动了蛋白质组学的研究。蛋白质组学为疾病发病机制的研究提供了新的思路和方法 ,本文重点介绍了蛋白质组学技术在心血管疾病研究中的应用     

蛋白质组学分析技术在微生物研究中的应用

随着后基因组时代的到来,蛋白质组学分析为研究微生物的生命活动和细胞功能提供了一个广阔的视角。综述了大规模分析微生物蛋白质组的策略和方法,包括自上而下的蛋白质组学分析、自下而上的蛋白质组学分析、蛋白质组定量分析技术、蛋白质修饰研究方法和蛋白质芯片技术。最后,对沙门氏菌蛋白质组学的研究进展进行了简要介绍。     

现代质谱技术在蛋白质组学中的应用及其最新进展

简述了蛋白质组学的概念、内容和意义,重点综述了现代质谱技术在蛋白质组学中的应用,主要包括蛋白质和肽段的鉴定和定量、蛋白质翻译后修饰的鉴定和蛋白质间相互作用的检测等。随着新的高质量精确度、分辨率、灵敏度和通量质谱仪的出现,现代质谱技术在蛋白质组学中的应用将越来越广泛,并给蛋白质组学研究带来新的机遇。     

Strategies for the enrichment and identification of basic proteins in proteome projects

Two-dimensional gel electrophoresis (2-DE) is currently the method of choice for separating complex mixtures of proteins for visual comparison in proteome analysis. This technology, however, is biased against certain classes of proteins including low abundance and hydrophobic proteins. Proteins with extremely alkaline isoelectric points (pI) are often very poorly represented using 2-DE technology, even when complex mixtures are separated using commercially available pH 6-11 or pH 7-10 immobilized pH gradients. The genome of the human gut pathogen, Helicobacter pylori, is dominated by genes encoding basic proteins, and is therefore a useful model for examining methodology suitable for separating such proteins. H. pylori proteins were separated on pH 6-11 and novel pH 9-12 immobilized pH gradients and 65 protein spots were subjected to matrix-assisted laser desorption/ionization-time of flight mass spectrometry, leading to the identification of 49 unique proteins. No proteins were characterized with a theoretical pI of greater than 10.23. A second approach to examine extremely alkaline proteins (pI > 9.0) utilized a prefractionation isoelectric focusing. Proteins were separated into two fractions using Gradiflow technology, and the extremely basic fraction subjected to both sodium dodecyl sulphate-polyacrylamide gel electrophoresis and liquid chromatography (LC) - tandem mass spectrometry post-tryptic digest, allowing the identification of 17 and 13 proteins, respectively. Gradiflow separations were highly specific for proteins with pI > 9.0, however, a single LC separation only allowed the identification of peptides from highly abundant proteins. These methods and those encompassing multiple LC 'dimensions' may be a useful complement to 2-DE for 'near-to-total' proteome coverage in the alkaline pH range.     

融合标签技术在膜蛋白结构研究中的应用

膜蛋白高级结构的研究包括不同的层次,即膜蛋白拓扑学结构的研究、利用核磁共振技术和蛋白质晶体衍射技术对三维结构的研究,以及膜蛋白复合体的研究。在研究过程中,如果能够基于膜蛋白的拓扑学结构预测,选择合适的蛋白质或多肽融合标签,利用基因融合技术在基因水平上对膜蛋白进行改造,可以产生含有融合标签的重组膜蛋自,不仅具有原有膜蛋白的功能活性,还具有融合标签所特有的生理生化特性,将会极大地促进膜蛋白结构和功能的研究。我们就目前膜蛋白结构研究中所涉及的融合标签技术及其应用策略和所取得的进展做一简述。     

Analyzing proteome topology and function by automated multidimensional fluorescence microscopy

Temporal and spatial regulation of proteins contributes to function. We describe a multidimensional microscopic robot technology for high-throughput protein colocalization studies that runs cycles of fluorescence tagging, imaging and bleaching in situ. This technology combines three advances: a fluorescence technique capable of mapping hundreds of different proteins in one tissue section or cell sample; a method selecting the most prominent combinatorial molecular patterns by representing the data as binary vectors; and a system for imaging the distribution of these protein clusters in a so-called toponome map. By analyzing many cell and tissue types, we show that this approach reveals rules of hierarchical protein network organization, in which the frequency distribution of different protein clusters obeys Zipf's law, and state-specific lead proteins appear to control protein network topology and function. The technology may facilitate the development of diagnostics and targeted therapies.     

Cloning of Fish Enzymes and Other Fish Protein Genes

ABSTRACT:?

Fish metabolism needs special enzymes that have maximum activity at very different conditions than their mammalian counterparts. Due to the differences in activity, these enzymes, especially cold-adapted proteases, could be used advantageously for the production of some foods. In addition to the enzymes, this review describes some other unique fish polypeptides such as antifreeze proteins, fluorescent proteins, antitumor peptides, antibiotics, and hormones, that have already been cloned and used in food processing, genetic engineering, medicine, and aquaculture. Recombinant DNA technology, which allows these biological molecules to be cloned and overexpressed in microorganisms is also described, highlighting innovative applications. The expected impact of cloning fish proteins in different fields of technology is discussed.     

The Human Proteome Organization Plasma Proteome Project pilot phase: reference specimens, technology platform comparisons, and standardized data submissions and analyses

A comprehensive, systematic characterization of cirolating proteins in health and disease will greatly facilitate development of biomarkers for prevention, diagnosis, and therapy of cancers and other diseases. The Human Proteome Organization Plasma Proteome Project pilot phase aims to (1) compare the advantages and limitations of many technology platforms; (2) contrast reference specimens of human plasma (ethylenediaminetetra acetic acid, heparin, citrate-anticoagulated) and serum, in terms of numbers of proteins identified and any interferences with various technology platforms; and (3) create a global knowledge base/data repository.     

Protein microarrays: promising tools for proteomic research

Miniaturized and parallelized ligand binding assays are of great interest in postgenomic research because microarray technology allows the simultaneous determination of a large number of parameters from a minute amount of sample within a single experiment. Assay systems based on this technology are used for the identification and quantification of proteins as well as for the study of protein interactions. Protein affinity assays have been implemented that allow the analysis of interactions between proteins with other proteins, peptides, low molecular weight compounds, oligosaccharides or DNA. Microarray technology is an emerging technology used in global analytical approaches and has a considerable impact on proteomic research.     

Heterologous protein production in yeast

The exploitation of recombinant DNA technology to engineer expression systems for heterologous proteins represented a major task within the field of biotechnology during the last decade. Yeasts attracted the attention of molecular biologists because of properties most favourable for their use as hosts in heterologous protein production. Yeasts follow the general eukaryotic posttranslational modification pattern of expressed polypeptides, exhibit the ability to secrete heterologous proteins and benefit from an established fermentation technology. Aside from the baker's yeastSaccharomyces cerevisiae, an increasing number of alternative non-Saccharomyces yeast species are used as expression systems in basic research and for an industrial application.In the following review a selection from the different yeast systems is described and compared.     

Prospects for the Application of Yeast Display in Biotechnology and Cell Biology (Review)

The technology of the yeast cell surface display, which appeared 20 years ago and was based on the displaying of target proteins on the cell surface via fusion to an abundant cell wall protein finds broad application in basic and applied research. The main advantage of the cell surface display on the basis of eukaryotic microorganisms—yeast—is the opportunity for correct modification of mammalian proteins. The cell surface display is an important tool for the analysis and understanding of protein function and protein–protein interactions and for the screening of novel clones from peptide and protein libraries. This technology makes it possible to obtain cells with novel abilities, such as catalytic functions and affinity binding to valuable ligands, including rare and heavy metals. It provides the chance to use yeast in biotechnology and in bioremediation and biomonitoring of the environment. The review considers the methods of obtaining a cell surface display on the basis of the yeasts Saccharomyces cerevisiae, Pichia pastoris, and Yarrowia lipolytica, the properties of anchor proteins, and the main fields of yeast display technology.     

Proteomic analysis of the mosquito Aedes aegypti midgut brush border membrane vesicles

We analyzed brush border membrane vesicle proteins from isolated midguts of the mosquito Aedes aegypti, by two proteomic methods: two-dimensional gel electrophoresis (isoelectric focusing and SDS-PAGE) and a shotgun two-dimensional liquid chromatographic (LS/LS) approach based on multidimensional protein identification technology (MudPIT). We were interested in the most abundant proteins of the apical brush border midgut membrane. About 400 spots were detected on 2D gels and 39 spots were cored and identified by mass spectrometry. 86 proteins were identified by MudPIT. Three proteins, arginine kinase, putative allergen and actin are shown to be the most predominant proteins in the sample. The total number of 36 proteins detected by both methods represents the most abundant proteins in the BBMV.     

Serum profile in preeclampsia and intra-uterine growth restriction revealed by iTRAQ technology

In order to identify new protein markers modified in placental diseases, high-throughput analysis of proteins in the plasma of pregnant women was carried out for normal and pathological pregnancies (Preeclampsia and/or Intra-Uterine Growth Restriction) using iTRAQ technology. We could identify 166 proteins that were modified (p < 0.05) and the technique used allowed the detection of previously undetected factors, such as various members of the SERPINA clade. The modifications of two proteins (C reactive protein and antichymotrypsin, SERPINA3) were validated on individual samples. Complement and coagulation cascades proteins were significantly enriched among modified protein clusters in the case of intra-uterine growth restriction (p < 2.6 · 10^? 11). Several proteins were specifically enriched in isolated preeclampsia and depleted when preeclampsia was complicated by intra-uterine growth restriction. These findings suggest that the growth restricted foeto-placental unit is able to moderate some changes in maternal plasma composition. Overall, the use of iTRAQ technology, for the first time on this subject, enabled us to provide a new list of proteins modified in placental diseases, among which proteins expressed at a low level that were not accessible by other methods.