Greening David W, Ji Hong, Kapp Eugene A, Simpson Richard J
La Trobe Institute for Molecular Science (LIMS), La Trobe University, Bundoora, Victoria, Australia.
Biochim Biophys Acta. 2013 Nov;1834(11):2293-307. doi: 10.1016/j.bbapap.2013.07.007. Epub 2013 Jul 27.
Colorectal cancer (CRC) is a major cause of mortality in Western populations. Growing evidence from human and rodent studies indicate that nonsteroidal anti-inflammatory drugs (NSAIDs) cause regression of existing colon tumors and act as effective chemopreventive agents in sporadic colon tumor formation. Although much is known about the action of the NSAID sulindac, especially its role in inducing apoptosis, mechanisms underlying these effects is poorly understood. In previous secretome-based proteomic studies using 2D-DIGE/MS and cytokine arrays we identified over 150 proteins released from the CRC cell line LIM1215 whose expression levels were dysregulated by treatment with 1mM sulindac over 16h; many of these proteins are implicated in molecular and cellular functions such as cell proliferation, differentiation, adhesion, angiogenesis and apoptosis (Ji et al., Proteomics Clin. Appl. 2009, 3, 433-451). We have extended these studies and describe here an improved protein/peptide separation strategy that facilitated the identification of 987 proteins and peptides released from LIM1215 cells following 1mM sulindac treatment for 8h preceding the onset of apoptosis. This peptidome separation strategy involved fractional centrifugal ultrafiltration of concentrated cell culture media (CM) using nominal molecular weight membrane filters (NMWL 30K, 3K and 1K). Proteins isolated in the >30K and 3-30K fractions were electrophoretically separated by SDS-PAGE and endogenous peptides in the 1-3K membrane filter were fractioned by RP-HPLC; isolated proteins and peptides were identified by nanoLC-MS-MS. Collectively, our data show that LIM1215 cells treated with 1mM sulindac for 8h secrete decreased levels of proteins associated with extracellular matrix remodeling (e.g., collagens, perlecan, syndecans, filamins, dyneins, metalloproteinases and endopeptidases), cell adhesion (e.g., cadherins, integrins, laminins) and mucosal maintenance (e.g., glycoprotein 340 and mucins 5AC, 6, and 13). A salient finding of this study was the increased proteolysis of cell surface proteins following treatment with sulindac for 8h (40% higher than from untreated LIM1215 cells); several of these endogenous peptides contained C-terminal amino acids from transmembrane domains indicative of regulated intramembrane proteolysis (RIP). Taken together these results indicate that during the early-stage onset of sulindac-induced apoptosis (evidenced by increased annexin V binding, dephosphorylation of focal adhesion kinase (FAK), and cleavage of caspase-3), 1mM sulindac treatment of LIM1215 cells results in decreased expression of secreted proteins implicated in ECM remodeling, mucosal maintenance and cell-cell-adhesion. This article is part of a Special Issue entitled: An Updated Secretome.
结直肠癌(CRC)是西方人群死亡的主要原因。来自人类和啮齿动物研究的越来越多的证据表明,非甾体抗炎药(NSAIDs)可使现有的结肠肿瘤消退,并在散发性结肠肿瘤形成中作为有效的化学预防剂。尽管对NSAID舒林酸的作用,尤其是其在诱导细胞凋亡中的作用已了解很多,但对这些作用的潜在机制仍知之甚少。在先前基于分泌蛋白质组的蛋白质组学研究中,使用二维差异凝胶电泳/质谱(2D-DIGE/MS)和细胞因子阵列,我们鉴定出从CRC细胞系LIM1215释放的150多种蛋白质,其表达水平在1mM舒林酸处理16小时后发生失调;其中许多蛋白质与分子和细胞功能有关,如细胞增殖、分化、黏附、血管生成和细胞凋亡(Ji等人,《蛋白质组学临床应用》,2009年,3卷,433 - 451页)。我们扩展了这些研究,并在此描述一种改进的蛋白质/肽分离策略,该策略有助于鉴定在细胞凋亡开始前用1mM舒林酸处理8小时后从LIM1215细胞释放的987种蛋白质和肽。这种肽组分离策略涉及使用标称分子量膜过滤器(NMWL 30K、3K和1K)对浓缩细胞培养基(CM)进行分级离心超滤。在>30K和3 - 30K级分中分离的蛋白质通过SDS-PAGE进行电泳分离,在1 - 3K膜过滤器中的内源性肽通过反相高效液相色谱(RP-HPLC)进行分级分离;分离的蛋白质和肽通过纳升液相色谱-串联质谱(nanoLC-MS-MS)进行鉴定。总体而言,我们的数据表明,用1mM舒林酸处理8小时的LIM1215细胞分泌的与细胞外基质重塑(如胶原蛋白、基底膜聚糖、多配体蛋白聚糖、细丝蛋白、动力蛋白、金属蛋白酶和内肽酶)、细胞黏附(如钙黏蛋白、整合素、层粘连蛋白)和黏膜维持(如糖蛋白340和黏蛋白5AC, 6和13)相关的蛋白质水平降低。这项研究的一个显著发现是,用舒林酸处理8小时后细胞表面蛋白质的蛋白水解增加(比未处理的LIM1215细胞高40%);这些内源性肽中的几种含有来自跨膜结构域的C末端氨基酸,表明存在调节性膜内蛋白水解(RIP)。这些结果共同表明,在舒林酸诱导的细胞凋亡早期(通过膜联蛋白V结合增加、粘着斑激酶(FAK)去磷酸化和半胱天冬酶-3裂解来证明),用1mM舒林酸处理LIM1215细胞会导致与细胞外基质重塑、黏膜维持和细胞间黏附相关的分泌蛋白表达降低。本文是名为:更新的分泌蛋白质组的特刊的一部分。
