毛细管电泳-激光诱导荧光分析血清多胺的研究

为进一步探讨多胺的生物学作用,建立了毛细管电泳-激光诱导荧光(λ_ex=488 nm,λ_em=513 nm)分析血清多胺方法.在碱性介质中,多胺与荧光素异硫氰酸酯进行衍生化反应,硼酸盐(pH 8.6)作为运行缓冲液,运行电压20 kV,腐胺、精胺、精脒和1,6-己二胺（内标）在8 min内达到基线分离.考察了方法的线性范围、稳定性、检测限和方法的回收率等,方法具有样品处理简单,灵敏度高,速度快等特点.用于正常对照大鼠和肿瘤大鼠血清多胺的测定.结果提示：实验组肿瘤大鼠血清精胺和精脒水平显著高于正常对照大鼠和实验组未出现肿瘤大鼠血清精胺和精脒水平（P＜0.05）,正常对照组大鼠和实验组未出现肿瘤大鼠血清精胺和精脒水平间无显著性差异（P＞0.05）,各组间血清腐胺水平均无显著性差异（P＞0.05）.     

Combination of Micropreparative Capillary Electrophoresis and Matrix-Assisted Laser Desorption/Ionization Mass Spectrometry for Peptide Analysis

Signal suppression is a problem in matrix-assisted laser desorption/ionization mass spectrometry of peptides prepared by capillary electrophoresis. Many common electrolytes that are efficient for separation, such as sodium phosphate, also are strongly suppressive during laser desorption/ionization. We have tested individual electrolytes for highest performance in each step of separation and collection, respectively. Suppression is not observed if citrate, trifluoroacetic acid, or hydrochloric acid is used for collection, while phosphate still can be employed in the capillary providing excellent resolution. Low concentrations of hydrochloric acid added to the sample/matrix mixture generate mass spectra with better ion intensities than if trifluoroacetic acid or citrate is used.     

单链构象多态性毛细管电泳分析研究进展

基因突变的检测在临床疾病诊断中起十分重要的作用.单链构象多态性(Single Strand Conform ationPolym orphism,SSCP)分析是检测突变最流行的方法之一.SSCP分析与毛细管电泳(Capillary Electrophoresis,CE)相结合的技术更是具有灵敏度高、花费低、简单、快速的优点.目前,这项技术已应用于人类原癌基因、抑癌基因以及其它致病基因的突变检测.主要综述了各种参数对CES-SCP分析的影响以及CES-SCP分析技术将来的发展方向.     

毛细管区带电泳／串联质谱联用法鉴定多肽和蛋白质

建立了毛细管区带电泳－串联质谱联用（ＣＺＥ／ＭＳ／ＭＳ）对多肽和蛋白质高灵敏度鉴定方法,对Ｍｅｔ－脑啡肽和Ｌｅｕ－脑啡肽的混合物进行了分析,用ＣＺＥ／ＭＳ／ＭＳ方法验证了各自的序列,同样对细胞色素ｃ的胰蛋白酶酶解产物用ＣＺＥ／ＭＳ／ＭＳ方法进行了肽质谱分析,几科所有肽段的序列及其与在分子中的位置都得到了确定,通过ＳＥＱＵＥＳＴ软件进行蛋白质序列数据库搜索得到准确的鉴定结果,所消耗的样品量均在低皮可     

引起重组白蛋白电泳检测假性结果的研究

目的:建立SDS-PAGE结合pH值变化对重组人血白蛋白电泳检测假性结果的分析方法。方法:采用还原SDS-PAGE(12.5%)和Native-PAGE(8%～25%),将包含重组人血白蛋白的发酵上清液的pH值分别调为4.0、5.0、6.0、6.5、7.5、8.0、9.0和10.0进行电泳分析。结果:在不同的pH值条件下,重组人血白蛋白会出现不同程度的降解。结论:包含重组人血白蛋白的发酵液中存在不同种类的蛋白酶,导致重组人血白蛋白的假性降解。     

毛细管电泳飞摩尔水平分析糖蛋白中唾液酸

利用毛细管电泳分析唾液酸2-氨基吖啶酮(AMAC)衍生物方法, 可在飞摩尔水平分析糖蛋白中唾液酸. 重组人促红细胞生成素(rhu-EPO)、人尿胰蛋白酶抑制剂(hu-UTI)中唾液酸分析结果与文献值符合较好; 而牛α₁-酸性糖蛋白(α₁-AGP)分析结果与早期文献值相比, 存在一定差异, 并发现该糖蛋白中除含有5-N-乙酰氨基唾液酸(Neu5Ac)外, 还含数量与Neu5Ac相当的5-N-乙醇酰氨基唾液酸(Neu5Gc).     

适于小麦叶片蛋白质组分析的样品提取方法研究

以‘铭贤169'小麦苗期叶片为材料,分别采用传统的TCA/丙酮沉淀法、酚提取-甲醇/醋酸铵沉淀法以及改进的TCA/丙酮沉淀-酚/SDS联合抽提法提取叶片总蛋白,进行双向电泳分离和胶体考染,以建立适用于小麦蛋白质组分析的样品制备方法.结果表明:TCA/丙酮沉淀法较酚提取-甲醇/醋酸铵沉淀法获得的蛋白杂质较少,在二维电泳图谱中的蛋白点较酚抽提-甲醇/醋酸铵沉淀法提取的蛋白点清晰且多.相比于以上2种提取蛋白样品方法,改进的TCA/丙酮沉淀-酚/SDS联合抽提法提取的小麦叶片蛋白杂质少、二维电泳图谱上的点明显增多、分辨率较高.所选小麦的代表性蛋白点能获得成功鉴定.该方法可推广应用于水稻叶片蛋白质组分析的样品提取.     

苦参碱的反胶束萃取研究

本文探索AOT-异辛烷反胶束萃取苦参碱的最佳工艺和条件,以AOT-异辛烷反胶束对粗苦参碱中的苦参碱进行萃取,利用毛细管电泳对苦参碱进行定量分析,通过正交试验优化萃取工艺和条件,确定影响萃取率的主要因素为萃取水相的酸度,次要因素为水相的温度,反胶束的W0和离子强度对萃取率的影响较小,得出最优萃取条件为:pH=12,W0=30,T=35℃。     

天花粉蛋白胰酶肽图谱的毛细管区带电泳法分析

目的:以天花粉蛋白胰蛋白酶解肽段为测定对象,用毛细管区带电泳法(CZE)研究天花粉蛋白的肽图谱分离条件。方法:采用未涂层石英毛细管(长50cm,内径75μm,有效长度42cm),以50mmol/L磷酸盐和150mmol/L三氟乙酸溶液为运行缓冲液,在25℃、pH2.0和压力为3447.4Pa(×10s)的条件下进样,以12kV恒压电泳分离,检测波长214nm。结果:运用CZE也能较好地对天花粉蛋白进行肽图谱分离,在缓冲体系中加入离子对试剂三氟乙酸,可极大地改善多肽的峰形和分辨率;同时运用反相高效液相色谱(RP-HPLC)技术,也很好地鉴定了部分肽段在CZE和RP-HPLC肽图谱中的对应关系。结论:与传统的RP-HPLC分析天然或重组蛋白肽图谱相比,CZE也不失为一种鉴定蛋白肽图谱的有效、快速和简单的方法。     

Assessment and Refinement of Sample Preparation Methods for Deep and Quantitative Plant Proteome Profiling

A major challenge in the field of proteomics is obtaining high‐quality peptides for comprehensive proteome profiling by LC–MS. Here, evaluation and modification of a range of sample preparation methods using photosynthetically active Arabidopsis leaf tissue are done. It was found that inclusion of filter‐aided sample preparation (FASP) based on filter digestion improves all protein extraction methods tested. Ultimately, a detergent‐free urea‐FASP approach that enables deep and robust quantification of leaf and root proteomes is shown. For example, from 4‐day‐old leaf tissue, up to 11 690 proteins were profiled from a single sample replicate. This method should be broadly applicable to researchers working with difficult to process plant samples.     

Comparative Proteome Analysis of Human Temporal Cortex Lobes by Two-Dimensional Electrophoresis and Identification of Selected Common Proteins

Human brain proteins were isolated from left and right temporal cortex lobes at the age of 73, 23, 84 years and separated by two-dimensional gel electrophoresis (2-DE). 2-DE was carried out with an immobilized pH gradient strip in the first dimension and by sodium dodecyl sulfate-polyacrylamide gel electrophoresis in the second dimension. Over 800 polypeptide spots were resolved with a silver-staining protocol by computerized 2-D gel analsis. Seven of the polypeptide spots were evidently distinguishable between human left and right temporal lobes. Four of the polypeptide spots were larger and three were smaller in human right temporal lobe. One of these three protein spots that have descendent expression in human right temporal lobe was identified as carbonyl reductase (NADPH) 1 by MALDI-TOF MS. Thirty-three common spots were identified by ESI-MS/MALDI-TOF MS/Edman sequencing and a protein database search. These identified proteins include some important enzymes and regulating proteins.     

毛细管电泳在细菌分离分析中的应用

介绍了近年来毛细管电泳技术在细菌分离分析方面的研究进展。毛细管电泳以细菌表面的特征信息为分离的基础,可以快速鉴定相应的菌株,可以对微生物进行快速定量,可以反映细菌特殊时期的生理特征,也可以研究微生物与分子之间的相互作用。同时应用该技术可分离分析自然界不能纯培养的微生物。因而毛细管电泳分离与检测细菌方法的建立及其应用在分离科学和微生物学方面都有很大的实际意义。     

二维电泳和质谱技术鉴定肝癌血清差异表达的N-连接糖蛋白

缺乏有效的早期诊断方法是导致肝细胞癌(hepatocellular carcinoma, HCC)预后极差的主要原因之一.蛋白质异常糖基化与恶性肿瘤细胞侵袭、转移等生物学过程关系密切,人体内至少有50%的蛋白质发生了糖基化修饰.本实验采用IgY12去除血清高丰度蛋白、多植物凝集素亲和层析技术分别从20例肝癌和年龄、性别匹配的20例非癌慢性肝病患者血清中纯化N 连接糖蛋白、二维电泳分析差异表达的蛋白质斑点,质谱检测、生物信息学等技术鉴定了18个差异表达的糖蛋白和/或其异质体（12种高表达和6种低表达）.ExPASy数据库比对结果表明,本实验鉴定的糖蛋白质分子含有至少1个已报道的N 糖基化位点.这些差异表达的糖蛋白属于急性期反应蛋白,分别具有蛋白酶抑制、生物转运、凝血和纤溶等功能,表明肝癌的发生发展过程中机体产生的急性期反应物可能是潜在的肝癌血清标志物.     

Enantioseparation of Tröger's Base Derivatives by Capillary Electrophoresis Using Cyclodextrins as Chiral Selectors

The enantioseparation of seven Tröger's base derivatives (TBs) was carried out by capillary electrophoresis using α‐, β‐, and γ‐cyclodextrins as chiral selectors and phosphate at 20 mmol/l concentration, pH 2.5, as background electrolyte. The method was optimized with respect to the concentration of chosen chiral selectors (0–50 mmol/l) and the amount of organic solvent (acetonitrile, 0–25 % (v/v)) in the electrolyte. The results indicate that all the studied variables, i.e., type of chiral selector, its concentration, and the amount of the added organic solvent, have a significant impact on the enantioseparation of the studied TBs. The best results for the majority of the separated TBs were obtained utilizing β‐cyclodextrin at 5 mmol/l concentration and with various amounts of acetonitrile added ranging from 5 to 15% (v/v) in the background electrolyte. For the two smallest studied TBs, γ‐cyclodextrin with 10% (v/v) acetonitrile also provided good resolution. Chirality 25:379–383, 2013. © 2013 Wiley Periodicals, Inc.     

Analysis of fluorescently labeled oligosaccharides by capillary electrophoresis and electrospray ionization mass spectrometry

Neutral oligosaccharides were fluorescently conjugated with 7-amino-1, 3-naphthalenedisulfonic acid. A mixture of fluorescently labeled chitobiose, chitotriose, and chitotetrose were successfully separated by preparative capillary electrophoresis (CE) and the individual components characterized by electrospray ionization-mass spectrometry (ESI-MS). By combining fluorescent labeling with CE, the use of highly specific exoglycosidases and ESI-MS, a more structurally complex N-linked glycan was analyzed.     

血浆蛋白质组——人类蛋白质组计划的“探路者”

概述了血浆蛋白的研究现状、难点和策略.血浆是血液中无形的液体成分,是一种十分复杂和多样化的基质,包含数百万种蛋白质和小分子多肽、盐、类脂、氨基酸和糖等.血浆蛋白参与机体免疫、凝血-抗凝血、物质运输、营养和对生长信号调节等多种重要的生理功能.人体器官的病理变化可导致血浆蛋白在结构和数量上的改变,这种特征性的变化对疾病诊断和疗效监测具有十分重要的意义.然而,迄今为止人类对血浆蛋白的了解还十分有限,只有很少一部分血浆蛋白被用于常规的临床诊断.全面而系统地认识健康和疾病状态下血液循环中血浆蛋白的性质,会极大地加速对具有疾病诊断和治疗监测作用的血浆标志蛋白的研发.国际人类蛋白质组组织于2002年首先选择了血浆蛋白质组作为人类蛋白质组首期执行计划之一,其初期目标是：a.比较各种蛋白质组分析技术平台的优点和局限性;b.用这些技术平台分析人类血浆和血清的参考样本;c.建立人类血浆蛋白质组知识库.     

毛细管电泳分离寡糖衍生物及其电泳行为研究

将葡聚糖部分酸水解成寡糖混合物,经ＡＮＴＳ胺化还原衍生,在ｐＨ２．５、５０ｍｍｏｌ／Ｌ磷酸缓冲液（含或不含１０ｍｍｏｌ／Ｌ ＴＥＡ）中,以及在ｐＨ９．３、１００ｍｍｏｌ／Ｌ硼砂缓冲液中用毛细管电泳分离衍生物,分别得到１至２１和１至１８个聚合度的衍生物电泳梯度图谱。作出了准确定位的毛细管电泳双向电泳图。对电泳行为研究发现,在低ｐＨ磷酸电泳缓冲液中,衍生物相对电迁移率（μｅｐ）ｒ与（Ｍｒ＾－２／３）、     

Analysis of glycoprotein heterogeneity by capillary electrophoresis and mass spectrometry

Glycosylation is a complex posttranslational modification that can result in extensive heterogeneity for recombinant glycoproteins produced by eukaryotic systems. The carbohydrate moiety of a recombinant glycoprotein may affect the immunogenicity, half-life, bioactivity, and stability of a potential therapeutic product. Regulatory authorities such as the US Food and Drug Administration demand increasingly sophisticated carbohydrate analysis to ensure product characterization, batch-to-batch consistency, and stability. The advent of new technologies for analysis of biopolymers by capillary electrophoresis and mass spectrometry has revolutionized strategies for recombinant protein characterization. In particular, recent advances in matrix-assisted laser desorption/ionization and electrospray ionization mass spectrometry now permit relatively rapid and detaned assessment of glycoprotein and oligosaccharide structure. In this article, we describe some applications of capillary electrophoresis and mass spectrometry to monitor the glycosylation associated with a model recombinant glycoprotein, human interferon-γ.     

Use of Sulfated Cyclofructan 6 and Sulfated Cyclodextrins for the Chiral Separation of Four Basic Pharmaceuticals by Capillary Electrophoresis

Sulfated cyclofructan 6 (S‐CF6) and sulfated cyclodextrins (S‐α‐, β‐, γ‐CDs) are highly selective chiral selectors for the enantioseparation of basic solutes. In this study, S‐CF6 was introduced for the enantiomeric separation of four basic pharmaceuticals (including tamsulosin, tiropramide, bupivacaine, and norephedrine) by capillary electrophoresis (CE), and the enantiomeric separation performance was compared with S‐α‐, β‐, γ‐CDs. The effects of the chiral selector type, chiral selector concentration, operating voltage, and column temperature were examined and optimized. Excellent resolutions were obtained for all solutes on these chiral selectors. Chirality 25:735–742, 2013. © 2013 Wiley Periodicals, Inc.     

Large-scale Identification of N-linked Intact Glycopeptides in Human Serum using HILIC Enrichment and Spectral Library Search

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Highlights

• •This study proposed a spectral library search method to accurately identify N-linked glycopeptides in human serum through LC-MS/MS with pMatchGlyco software.
• •The identification depth of serum N-linked intact glycopeptides and glycoproteins was increased by combination of acetonitrile precipitation, HILIC enrichment and high-pH RPLC fractionation.
• •22,677 unique serum N-linked intact glycopeptides corresponding to 526 N-linked glycoproteins were identified with N-glycosylation motif-specific FDR control.
• •This study revealed the great microheterogeneity of N-linked glycoproteins in serum.