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Short Gel, Long Gradient Liquid Chromatography Tandem Mass Spectrometry to Discover Urinary Biomarkers of Chronic Pancreatitis. 短凝胶,长梯度液相色谱串联质谱法发现慢性胰腺炎尿液生物标志物。
Pub Date : 2013-01-01 DOI: 10.2174/1875039701306010001
Joao A Paulo, Vivek Kadiyala, Scott Brizard, Peter A Banks, Darwin L Conwell, Hanno Steen

Background: Chronic pancreatitis (CP) is currently diagnosed using invasive endoscopic as well as radiation and non-radiation-based imaging techniques. However, urine can be safely and non-invasively collected and as such may offer a superior alternative to current techniques of CP diagnosis. We use mass spectrometry-based methods to discover proteins which are exclusive to or differentially abundant in urine of chronic pancreatitis patients.

Methods: We have performed a comparative quantitative proteomic analysis of urine collected from 5 healthy controls and 5 severe CP patients. Proteins from urine were fractionated briefly on SDS-PAGE and subsequently digested in-gel with trypsin. The resulting peptides were fractionated for 3 hours by reversed-phase liquid chromatography in-line with a mass spectrometer. ProteinPilot software and the QSPEC algorithm identified proteins and determined statistically significant differences between cohorts. In addition, we used a third cohort of non-CP disease patients to filter out those proteins which may be indicative of an ailment other than CP.

Results: We identified over 600 proteins from urine, of which several hundred were either exclusive to or differ quantitatively between healthy controls and severe CP patients. Members of the cathepsin protein family were of significantly higher abundance in the severe CP cohort. In addition, we have identified a core set of 50 proteins in all 15 samples, 25 of which showed no significant difference among the cohorts.

Conclusions: Proteomic analysis identified differentially abundant proteins in healthy controls and severe CP patients. Such proteins represent an initial set of targets for directed proteomics experiments for further validation studies. However, larger cohorts will be required to determine if these differences have statistically significant diagnostic potential.

背景:慢性胰腺炎(CP)目前是通过侵入性内窥镜以及放射和非放射成像技术诊断的。然而,尿液可以安全、无创地收集,因此可能为目前的CP诊断技术提供更好的选择。我们使用基于质谱的方法来发现慢性胰腺炎患者尿液中独有或差异丰富的蛋白质。方法:对5例健康对照和5例重症CP患者的尿液进行比较定量的蛋白质组学分析。尿液中的蛋白质在SDS-PAGE上短暂分离,随后用胰蛋白酶凝胶消化。所得多肽经反相液相色谱联用质谱仪分离3小时。ProteinPilot软件和QSPEC算法识别蛋白质并确定队列之间的统计学显著差异。此外,我们使用了第三组非CP疾病患者来过滤掉可能指示CP以外疾病的蛋白质。结果:我们从尿液中鉴定出600多种蛋白质,其中数百种蛋白质在健康对照组和严重CP患者之间是专有的或在数量上不同。组织蛋白酶蛋白家族成员在严重CP队列中丰度明显更高。此外,我们在所有15个样本中鉴定了50个蛋白质的核心集,其中25个在队列中没有显着差异。结论:蛋白质组学分析发现,健康对照者和重症CP患者的蛋白质含量存在差异。这些蛋白质代表了定向蛋白质组学实验的初始目标,以进一步验证研究。然而,需要更大的队列来确定这些差异是否具有统计学意义的诊断潜力。
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引用次数: 8
Quantitative Proteomic Analysis of Formalin Fixed Paraffin Embedded Oral HPV Lesions from HIV Patients. 福尔马林固定石蜡包埋HIV患者口腔HPV病变的定量蛋白质组学分析。
Pub Date : 2008-01-01 DOI: 10.2174/1875039700801010040
Mohit Raja Jain, Tong Liu, Jun Hu, Marlene Darfler, Valerie Fitzhugh, Joseph Rinaggio, Hong Li

Human immunodeficiency virus (HIV) infection is associated with dysplastic changes in oral human papilloma virus (HPV) lesions, suggesting changes in keratinocytes. In the present study, we seek to identify proteomic changes in oral HPV lesions between HIV(+) and HIV(-) patients. While fresh tissues represent the most desirable samples for proteomic investigations, they are often difficult to obtain in large numbers under clinical settings. We therefore have developed a new method to identify protein changes in formalin fixed and paraffin-embedded (FFPE) oral HPV lesions utilizing iTRAQ™ technology in conjunction with Liquid Tissue® sample preparation method. Using this method, we identified nine proteins that were differentially expressed in oral HPV lesions as a result of HIV infection. The quantitative proteomic method presented here will be valuable for others who plan to analyze FFPE tissues.

人类免疫缺陷病毒(HIV)感染与口腔人乳头瘤病毒(HPV)病变的发育异常变化有关,提示角化细胞发生变化。在本研究中,我们试图确定HIV(+)和HIV(-)患者口腔HPV病变的蛋白质组学变化。虽然新鲜组织是蛋白质组学研究中最理想的样本,但在临床环境下往往难以大量获得。因此,我们开发了一种利用iTRAQ™技术结合Liquid Tissue®样品制备方法来鉴定福尔马林固定和石蜡包埋(FFPE)口腔HPV病变中蛋白质变化的新方法。使用这种方法,我们鉴定了由于HIV感染而在口腔HPV病变中差异表达的9种蛋白质。这里提出的定量蛋白质组学方法将对其他计划分析FFPE组织的人有价值。
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引用次数: 39
Widespread Occurrence of Non-Enzymatic Deamidations of Asparagine Residues in Yersinia pestis Proteins Resulting from Alkaline pH Membrane Extraction Conditions. 由于碱性膜提取条件,鼠疫耶尔森菌蛋白中天冬酰胺残基的非酶脱酰胺现象广泛发生。
Pub Date : 2008-01-01 DOI: 10.2174/1875039700801010106
Moo-Jin Suh, Hamid Alami, David J Clark, Prashanth P Parmar, Jeffrey M Robinson, Shih-Ting Huang, Robert D Fleischmann, Scott N Peterson, Rembert Pieper

Extraction of crude membrane fractions with alkaline solutions, such as 100-200 mM Na(2)CO(3) (pH ~11), is often used to solubilize peripheral membrane proteins. Integral membrane proteins are largely retained in membrane pellets. We applied this method to the fractionation of membrane proteins of the plague bacterium Yersinia pestis. Extensive horizontal spot trains were observed in 2-DE gels. The pI values of the most basic spots part of such protein spot trains usually matched the computationally predicted pI values. Regular patterns of decreasing spot pI values and in silico analysis with the software ProMoST suggested ;n-1' deamidations of asparagine (N) and/or glutamine (Q) side chains for ;n' observed spots of a protein in a given spot train. MALDI-MS analysis confirmed the occurrence of deamidations, particularly in N side chains part of NG dipeptide motifs. In more than ten cases, tandem MS data for tryptic peptides provided strong evidence for deamidations, with y- and b-ion series increased by 1 Da following N-to-D substitutions. Horizontal spot trains in 2-DE gels were rare when alkaline extraction was omitted during membrane protein sample preparation. This study strongly supports the notion that exposure to alkaline pH solutions is a dominant cause of extensive N and Q side chain deamidations in proteins during sample preparation of membrane extracts. The modifications are of non-enzymatic nature and not physiologically relevant. Therefore, quantitative spot differences within spot trains in differential protein display experiments following the aforementioned sample preparation steps need to be interpreted cautiously.

用碱性溶液萃取粗膜馏分,如100- 200mm Na(2)CO(3) (pH ~11),常用于外周膜蛋白的溶解。整体膜蛋白大部分保留在膜颗粒中。我们将该方法应用于鼠疫耶尔森氏菌膜蛋白的分离。在2-DE凝胶中观察到广泛的水平斑点序列。这种蛋白质斑点序列的最基本斑点部分的pI值通常与计算预测的pI值相匹配。斑点pI值下降的规律和ProMoST软件的硅分析表明,在给定的斑点序列中,对观察到的蛋白质的N '个斑点,天冬酰胺(N)和/或谷氨酰胺(Q)侧链进行N -1'脱酰胺。MALDI-MS分析证实了脱酰胺的发生,特别是在NG二肽基序的N侧链部分。在十多个案例中,色氨酸的串联质谱数据提供了脱酰胺的有力证据,在N-to-D取代后,y-和b-离子系列增加了1da。当膜蛋白样品制备过程中省略碱性提取时,2-DE凝胶中很少出现水平斑点序列。这项研究有力地支持了这样一种观点,即在膜提取物的样品制备过程中,暴露于碱性pH溶液是蛋白质中广泛的N和Q侧链脱酰胺的主要原因。这些修饰是非酶促性质的,与生理无关。因此,根据上述样品制备步骤,需要谨慎解释差异蛋白展示实验中斑点序列内的定量斑点差异。
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引用次数: 6
Quantification of Serum Proteins of Metastatic Oral Cancer Patients Using LC-MS/MS and iTRAQ Labeling. 使用LC-MS/MS和iTRAQ标记定量口腔癌转移患者血清蛋白。
Pub Date : 2008-01-01 DOI: 10.2174/1875039700801010072
Lifeng Zhang, Jiang Jiang, Martha Arellano, Lei Zhang, Xinmin Yan, David T Wong, Shen Hu

Metastasis is a critical event in oral squamous cell carcinoma (OSCC) progression. In this study, we have performed quantitative analysis of serum proteins from non-metastatic (lymph-node metastasis free) and metastatic OSCC patients using liquid chromatography-tandem mass spectrometry (LC-MS/MS) with iTRAQ labeling (isobaric tagging for relative and absolute quantitation). To eliminate highly abundant proteins, the serum samples were initially separated by SDS-PAGE and only low abundant protein bands were excised for subsequent in-gel tryptic digestion. The resulting peptides were then extracted from each sample gels and labeled with iTRAQ reagent 114 (control), 116 (non-metastatic) and 117 (metastatic), respectively. Afterwards, the labeled samples were combined and subjected to LC-MS/MS analysis using linear ion trap (LIT) MS with pulsed Q collision induced dissociation (PQD). A total of 64 proteins were identified and quantified by this approach. Our study showed that iTRAQ labeling and LIT-MS with PQD is a valuable approach to quantification of serum proteins. We also demonstrated the presence of differentially expressed serum proteins between non-metastatic and metastatic OSCCs that may be further validated as biomarkers for metastatic OSCC. However, in order to comprehensively quantify low abundant serum proteins, a more efficient approach is needed to deplete highly abundant proteins prior to quantitative serum proteome analysis of OSCC.

转移是口腔鳞状细胞癌(OSCC)进展中的一个关键事件。在这项研究中,我们使用液相色谱-串联质谱(LC-MS/MS)对非转移性(无淋巴结转移)和转移性OSCC患者的血清蛋白进行了定量分析,并使用iTRAQ标记(相对和绝对定量等压标记)。为了消除高丰度的蛋白质,首先用SDS-PAGE分离血清样品,只切除低丰度的蛋白质带,用于随后的凝胶内胰蛋白酶消化。然后从每个样品凝胶中提取所得肽,分别用iTRAQ试剂114(对照)、116(非转移)和117(转移)标记。然后,将标记的样品组合,并使用线性离子阱(LIT) MS与脉冲Q碰撞诱导解离(PQD)进行LC-MS/MS分析。该方法共鉴定和定量了64个蛋白。我们的研究表明,iTRAQ标记和PQD的LIT-MS是一种有价值的血清蛋白定量方法。我们还证明了非转移性OSCC和转移性OSCC之间存在差异表达的血清蛋白,这可能进一步被验证为转移性OSCC的生物标志物。然而,为了全面量化低丰度的血清蛋白,在定量分析OSCC血清蛋白质组学之前,需要一种更有效的方法来消耗高丰度的蛋白。
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引用次数: 12
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The open proteomics journal
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