干旱胁迫对不同抗旱性棉花品种抗氧化酶活性及基因表达的影响

为明确不同抗旱性棉花品种对干旱胁迫的适应性差异,该研究选用‘新陆早50号’(耐旱型)和‘新陆早27号’(干旱敏感型)为材料,分析干旱及复水处理下两材料的活性氧产生、电解质渗漏、抗氧化酶活性变化,并分析部分抗氧化酶基因、渗透调节基因和转录因子在干旱胁迫下的表达谱。结果显示:(1)棉花叶片的电导率和MDA含量随着干旱胁迫的加强逐渐增加,复水后恢复;在干旱胁迫处理6和8d,耐旱型品种‘新陆早50号’的抗氧化酶活性显著高于干旱敏感型品种‘新陆早27号’。(2)基因表达谱分析显示,棉花超氧化物歧化酶基因(GhSOD)仅在干旱胁迫下表达,且2个品种间差异不显著,GhBADH、GhNCED和GhP5Cs及转录因子GhPHD1、GhPHD5、GhPHD6和GhPHD10在‘新陆早50号’叶片中的表达量均高于‘新陆早27号’。研究表明,耐旱型棉花品种较干旱敏感型在干旱胁迫下其体内的活性氧含量、电导率和MDA含量较低,抗氧化酶活性较高,并且其抗旱相关基因表达量也更高。     

人工老化处理对结球甘蓝种子生理生化特性的影响

以结球甘蓝品种‘冬升’种子为材料,研究高温(40℃)高湿(相对湿度100%)人工老化处理过程中种子的萌发特性、种子浸出液相对电导率和丙二醛、可溶性蛋白、可溶性糖含量以及抗氧化酶活性的变化,以揭示种子劣变的机理。结果表明:(1)人工老化处理甘蓝种子的含水量和不正常苗率均随着老化时间的延长逐渐增加,而种子发芽势、发芽率、发芽指数和活力指数的增加均逐渐降低。(2)随着处理天数的延长,老化处理甘蓝种子的浸出液电导率显著增大,浸出液可溶性糖含量逐渐升高,可溶性蛋白含量表现出显著下降趋势,而种子MDA含量呈先升高后逐渐下降的趋势。(3)在结球甘蓝种子老化进程中,其种子中SOD、POD、CAT活性变化的趋势相似,均随老化程度的加深而逐渐降低;而APX活性在老化处理的最初2d显著增加,第6天显著降低。研究发现,在结球甘蓝种子老化进程中,种子活力和萌发率显著降低,其种子浸出液电导率、可溶性蛋白含量、可溶性糖含量、保护酶活性变化与种子老化及劣变程度密切相关,膜脂过氧化作用可能是引起或加剧种子老化劣变的重要原因之一。     

番茄幼苗盐胁迫响应蛋白质组分析

采用营养液栽培,以盐敏感型番茄品种M82为试材,利用双向电泳(2-DE)研究盐胁迫处理下幼苗叶片蛋白质的表达谱,并采用基质辅助激光解析飞行时间串联质谱(MALDI-TOF/TOF-MS)技术进行差异蛋白质的分离及质谱鉴定。结果表明:(1)盐胁迫处理下,利用2-DE获得差异显著蛋白点20个,其中17个蛋白质点丰度上调表达,3个蛋白质点丰度下调表达。(2)通过质谱分析和蛋白质NCBInr数据库检索,共鉴定出19个差异蛋白,分别为果糖-二磷酸醛缩酶、S-腺苷甲硫氨酸合成酶、甘油醛-3-磷酸脱氢酶等及3个功能未知蛋白;这些鉴定出的差异蛋白质与能量代谢、光合作用、蛋白合成、氧化还原平衡等过程相关,暗示所分离鉴定的蛋白可能参与了番茄的盐胁迫响应,为进一步研究番茄抗逆机制奠定基础。     

‘培矮64S’与其eui突变体‘长选3S’穗颈节间蛋白质组差异分析

为从蛋白质表达水平了解长穗颈温敏核不育水稻穗颈节间伸长机理,该研究以长穗颈(EUI)温敏核不育水稻‘长选3S’为材料,温敏核不育水稻‘培矮64S’为对照,采用固相pH梯度双向凝胶电泳和质谱分析方法,对2个水稻材料抽穗前2 d的穗颈节间蛋白质进行分离,并进行差异蛋白质组学的比较研究。结果表明:(1)获得了分辨率和重复性较好的双向凝胶电泳图谱。(2)对40个差异蛋白质点进行MALDI-TOF-TOF-MS肽质谱指纹图谱分析,成功鉴定其中27个差异蛋白质点;与‘培矮64S’相比,‘长选3S’中有17个上调表达和10个下调表达的蛋白质。(3)差异蛋白质按照其功能可分为6类,其中主要是与细胞代谢相关蛋白,其次是与细胞壁重建相关蛋白;并且这些差异蛋白质可能与‘长选3S’抽穗期穗颈节间剧烈伸长生长有关,尤其是细胞壁重建相关蛋白与细胞的伸长密切相关。(4)实时荧光定量PCR对随机挑选的蛋白点2、7、8、24、35和36所对应的基因在两个材料最上节间的表达结果显示,‘长选3S’的2(Os10g08550)、7(Os12g42876)、8(Os01g55830)基因的表达量较‘培矮64S’明显下调,而24(Os06g48760)、35(Os05g25850)、36(Os07g42300)基因的表达量较‘培矮64S’显著上调,表明q-PCR的结果与蛋白凝胶图分析结果一致。研究认为,水稻eui基因可能是通过调节抽穗期穗颈节间这些蛋白质的表达,从而促进穗颈节间细胞分裂,尤其是细胞的伸长生长。     

干旱胁迫下不同抗旱水平陆地棉的叶片蛋白质组学比较研究

为了探讨陆地棉品种抗旱机理,以陆地棉抗旱品种‘中H177’和不抗旱品种‘中S9612’为材料,运用双向电泳结合质谱技术,分析干旱胁迫下不同陆地棉三叶期叶片蛋白质组分差异变化。结果表明:干旱胁迫下,不同陆地棉叶片蛋白表达差异较大;‘中H177’出现30个差异表达蛋白质点,‘中S9612’出现47个差异表达蛋白质点,只在‘中H177’表达差异的蛋白点11个,只在‘中S9612’表达差异的蛋白点28个,差异表达一致蛋白点8个,表达不一致蛋白点11个。质谱共鉴定出43个差异表达蛋白;功能分类分析表明,干旱胁迫蛋白参与光合作用、物质与能量代谢、抗逆相关蛋白、物质运输和活性氧清除;Rubisco活化酶和能量代谢相关蛋白ATP合成酶类表达差异最大。研究结果可以初步为陆地棉抗旱机理的探讨提供一定的理论基础。     

强休眠玉米种子休眠前后的蛋白差异表达

以强休眠玉米自交系08-641为试验材料,分别对处于休眠状态下的新鲜收获种子和经过10 d后熟作用破除休眠的种子进行了蛋白质组学差异表达分析。结果表明,通过双向电泳技术在3次重复试验下休眠状态的08-641鲜种子蛋白2-DE图谱上共检测到约600个蛋白质点,在经过10 d后熟作用破除休眠的08-641种子蛋白2-DE图谱上共检测到约620个蛋白质点,其中下调表达蛋白质点4个,上调表达蛋白质点4个,新增蛋白质点8个,缺失表达蛋白质点7个。经过质谱鉴定的差异表达蛋白质主要涉及球蛋白、胚胎晚期丰富蛋白、豆球蛋白等贮藏物蛋白质;蛋白酶体、山梨醇脱氢酶等参与物质代谢的蛋白质;热激蛋白等参与蛋白质结构、细胞功能调控的蛋白质。推测08-641种子休眠是由于种子内休眠相关蛋白的过量表达或缺失抑制了种子的正常萌发。     

棉花两品种耐盐性与抗氧化能力的相关性

对‘新陆早17’和‘中棉49’两个棉花（Gossypium hirsutumL.）品种在氧化剂甲基紫精（MV）和NaCl胁迫下的生理应答进行了研究,以期阐明棉花抗氧化能力与耐盐性的关系。研究结果表明,在40μmol·L-1MV胁迫3d,‘新陆早17’的丙二醛（MDA）和活性氧含量比‘中棉49’低,而抗坏血酸（AsA）、超氧化物岐化酶（SOD）、过氧化氢酶（CAT）和抗坏血酸过氧化物酶（APX）活性则高于‘中棉49’,表明‘新陆早17’抗氧化能力更强。在200mmol·L-1NaCl胁迫25d,‘新陆早17’的株高和叶绿素降低量、根部Na＋含量、相对电导率都低于‘中棉49’,说明‘新陆早17’耐盐更强。盐胁迫下‘新陆早17’的抗氧化酶活性上升而‘中棉49’却降低,表明‘新陆早17’通过上调SOD、CAT和APX活性来提高其耐盐性。结合棉花两品种的抗氧化和耐盐性差异,说明棉花抗氧化能力的高低能够影响品种的耐盐性。     

龙眼采后果肉劣变的差异表达蛋白分析

为探索龙眼(Dimocarpus longan)果肉常温劣变过程中蛋白质的变化, 采用蛋白质组学的方法, 在‘福眼’龙眼果肉常温劣变过程中发现共有24 个2 倍差异表达蛋白, 其中21 个蛋白被成功鉴定。这些蛋白参与了应激反应与防御(56%)、能量与碳代谢(19%)、初级代谢(5%)、蛋白转运(5%)和细胞骨架(5%)等细胞代谢活动。大多数与抗氧化作用密切相关的蛋白质都下调表达, 说明龙眼采后果肉的抗氧化能力有所下降, 不能有效地缓解ROS 积累引起的毒性作用, 从而使果肉劣变。此外, 与能量代谢相关的蛋白全部下调表达, 表明龙眼果实采后果肉劣变可能与能量供应不足有关。这些结果为龙眼采后保鲜技术研究提供科学依据。     

陆地棉‘徐州142’纤维不同发育时期蛋白质组比较分析

该研究以陆地棉‘徐州142’为材料,于开花后5、10、15、20、25、30d分别取样(棉铃)代表6个不同时期的棉纤维,利用双向电泳技术比较了棉纤维发育不同时期蛋白质组的变化,以明确不同发育阶段差异表达蛋白质及其功能与纤维发育之间的关系,为棉花产量和品质的改良提供理论依据。结果显示:(1)随着棉花的发育,棉纤维中的总蛋白含量逐渐降低,在开花后5d(5DPA)时棉花纤维中总蛋白的含量最高,达到11.7%,同时2-DE图谱中发现了15个明显的差异蛋白点;(2)运用MALDI-TOF-MS对差异蛋白质点鉴定结果发现,有5个明显的差异蛋白与棉花纤维发育相关,分别是GhSAM、GhPGK、GhCSD、GhFB和GhMDH蛋白;(3)开花后不同时期棉纤维蛋白质组的2-DE图谱表明,GhSAM、GhPGK1和GhMDH 3个蛋白在整个发育期都表达,但GhCSD从15DPA开始表达,GhFB从20DPA开始表达,而且GhSAM在15DPA时蛋白表达量最高,GhPGK1在10DPA时表达量最高,GhMDH、GhCSD和GhFB都是在30DPA时表达量最高。研究表明,棉纤维发育不同时期存在着差异蛋白,且在纤维发育不同时期蛋白的表达量也存在差异,同时这些差异蛋白参与能量代谢、碳代谢、细胞周期调控和发育等途径。     

氯沙坦对自发性高血压大鼠肾脏蛋白质表达谱的影响

目的:研究氯沙坦对自发性高血压大鼠肾脏组织蛋白质表达的影响。方法:采用蛋白质组学的技术,建立自发性高血压和氯沙坦干预后高血压大鼠肾脏的蛋白质二维凝胶电泳图谱,利用Imagemaster2Dv5.0软件分析蛋白点,并通过LC-MS/MS质谱分析和数据库检索鉴定差异蛋白质。结果:两组凝胶的平均蛋白点数分别为570±48、686±30。氯沙坦干预后有13个蛋白表达发生了显著变化,表达增强4个,表达降低4个,蛋白点消失5个。13个差异蛋白点进行质谱分析,鉴定出的7个蛋白质为Heat shock protein(Hsp)、Tubulin alpha-1chain、Transthyretin precursor、Liver regeneration-related protein LRRG03、Ezrin-radixin-moesin binding phosphoprotein50、Phosphoglycerate kinase1、Anionic trypsin I precursor。结论:这些差异表达的蛋白质可能在氯沙坦对高血压肾脏保护中发挥一定作用。     

Proteomic analysis of the venom of the predatory ant Pachycondyla striata (Hymenoptera: Formicidae)

The ants use their venom for predation, defense, and communication. The venom of these insects is rich in peptides and proteins, and compared with other animal venoms, ant venoms remain poorly explored. The objective of this study was to evaluate the protein content of the venom in the Ponerinae ant Pachycondyla striata. Venom samples were collected by manual gland reservoir dissection, and samples were submitted to two‐dimensional gel electrophoresis and separation by ion‐exchange and reverse‐phase high‐performance liquid chromatography followed by mass spectrometry using tanden matrix‐assisted laser desorption/ionization with time‐of‐flight (MALDI‐TOF/TOF) mass spectrometry and electrospray ionization‐quadrupole with time‐of‐flight (ESI‐Q/TOF) mass spectrometry for obtaining amino acid sequence. Spectra obtained were searched against the NCBInr and SwissProt database. Additional analysis was performed using PEAKS Studio 7.0 (Sequencing de novo). The venom of P. striata has a complex mixture of proteins from which 43 were identified. Within the identified proteins are classical venom proteins (phospholipase A, hyaluronidase, and aminopeptidase N), allergenic proteins (different venom allergens), and bioactive peptides (U10‐ctenitoxin Pn1a). Venom allergens are among the most expressed proteins, suggesting that P. striata venom has high allergenic potential. This study discusses the possible functions of the proteins identified in the venom of P. striata.     

MALDI TOF MS在细菌检测和鉴定中的应用

近年来质谱技术有了快速的发展,新的软电离技术,基质辅助激光解析电离和电喷雾电离使得质谱能够对核酸或蛋白质,多肽等生物大分子进行微量分析,且具有高灵敏度和高质量检测范围,通过串联质谱的分析还可以得到结构信息。MALDI TOF MS能给出微生物多方面的信息,包括分子量和结构信息等,用于微生物的各种研究中,如根据细菌的组成成分获得指纹图谱检测和鉴定细菌,细菌体内含有大量的生物标志分子能用于细菌的化学分类和鉴定。     

Sulfonation chemistry as a powerful tool for MALDI TOF/TOF de novo sequencing and post-translational modification analysis.

Mass spectrometry using matrix-assisted laser desorption/ionization (MALDI) is a widespread technique for various types of proteomic analysis. In the identification of proteins using peptide mass fingerprinting, samples are enzymatically digested and resolved into a number of peptides, whose masses are determined and matched with a sequence data-base. However, the presence inside the cell of several splicing variants, protein isoforms, or fusion proteins gives rise to a complex picture, demanding more complete analysis. Moreover, the study of species with yet uncharacterized genomes or the investigation of post-translational modifications are not possible with classical mass fingerprinting, and require specific and accurate de novo sequencing. In the last several years, much effort has been made to improve the performance of peptide sequencing with MALDI. Here we present applications using a fast and robust chemical modification of peptides for improved de novo sequencing. Post-source decay of derivatized peptides generates at the same time peaks with high intensity and simple spectra, leading to a very easy and clear sequence determination.     

Screening & analysis of anionic peptides from Foeniculum vulgare Mill by mass spectroscopy

Fennel (Foeniculum vulgare Mill.) member from the family Umbelliferae (Apiaceae) and has been used in Saudi Arabia as an medicine as of the from the tradition. Our previous work with seed extracts of this plant generated DEAE-ion exchange purified proteins that exhibited antibacterial properties. The current study moves this work forward by using 2-D gel separation and MALDI TOF/TOF to identify proteins in this active extract. Fourteen protein spots were excised, digested, and identified. Several putative functions were identified, including: a copper-trans locating ATPase PAA1 chloroplastic-like isoform X1; a cytosolic enolase; a putative pentatricopeptide repeat-containing protein; an NADP-requiring isocitrate dehydrogenase; two proteins annotated as being encoded downstream from Son-like proteins; three probable nuclear proteins 5–1; and four predicted/ unidentified proteins. Future efforts will further characterize their relevant antimicrobial properties with the aim of cloning and high throughput synthesis of the antimicrobial element(s).     

Intermittent administration of morphine alters protein expression in rat nucleus accumbens

Repeated exposure to drugs of abuse causes time-dependent neuroadaptive changes in the mesocorticolimbic system of the brain that are considered to underlie the expression of major behavioral characteristics of drug addiction. We used a 2-D gel-based proteomics approach to examine morphine-induced temporal changes in protein expression and/or PTM in the nucleus accumbens (NAc) of morphine-sensitized rats. Rats were pretreated with saline [1 mL/kg subcutaneously (s.c.)] or morphine (10 mg/kg, s.c.) once daily for 14 days and the animals were decapitated 1 day later. The NAc was extracted and proteins resolved by 2-DE. Several protein functional groups were found to be regulated in the morphine-treated group, representing cytoskeletal proteins, proteins involved in neurotransmission, enzymes involved in energy metabolism and protein degradation, and a protein that regulates translation.     

Improved protein sequence coverage by on resin deglycosylation and cysteine modification for biomarker discovery

Membrane proteins and secreted factors (soluble proteins or extracellular matrix components) are the targets of most monoclonal antibodies, which are currently in clinical development. These proteins are frequently post‐translationally modified, e.g. by the formation of disulfide bonds or by glycosylation, which complicates their identification using proteomics technologies. Here, we describe a novel methodology for the on resin deglycosylation and cysteine modification of proteins after in vitro, in vivo or ex vivo biotinylation. Biotinylated proteins are captured on streptavidin resin and all subsequent modifications, as well as the proteolytic digestion, which yields peptides for MS analysis, are performed on resin. Using biotinylated bovine fetuin‐A as a test protein, an improvement in sequence coverage from 7.9 to 58.7% could be shown, including the identification of all three glycosylation sites. Furthermore, a complex mixture derived from the ex vivo biotinylation of vascular structures in human kidney with cancer obtained by perfusion after surgical resection revealed almost a doubling of sequence coverage for all checked proteins when analyzed by LC‐MALDI TOF/TOF.     

Labeling elastase digests with TMT: informational gain by identification of poorly detectable peptides with MALDI-TOF/TOF mass spectrometry

The applicability of the less specific protease elastase for the identification of membrane and cytosolic proteins has already been demonstrated. MALDI as ionization technique particularly favors the detection of basic and to a lesser extent of weakly acidic peptides, whereas neutral peptides often remain undetected. Moreover, peptides below 700 Da are routinely excluded. In the following study, the advantage of additional information gained from tandem mass tag zero labeled peptides and the resultant increase in sequence coverage was evaluated. Through derivatization with tandem mass tag reagents, peptide measurement within the standard mass range of the MALDI reflector mode is achievable due to the mass increase. Compared to the unlabeled sample, peptides exhibiting relatively low molecular masses, pI values or higher hydrophobicity could be identified.