凋亡细胞新型富含α-D-甘露糖糖蛋白标志物的体内表达及特征

Bilyy Rostyslav, Kit Yuriy, Hellman Ulf, Tryndyak Volodymyr, Kaminskyy Vitaliy, Stoika Rostyslav

Institute of Cell Biology, National Academy of Sciences of Ukraine, Drahomanov Street 14/16, Lviv 79005, Ukraine.

Cell Biol Int. 2005 Nov;29(11):920-8. doi: 10.1016/j.cellbi.2005.08.003. Epub 2005 Oct 20.

We recently established that an increased expression of alpha-D-mannose (Man)- and beta-D-galactose-rich plasma membrane glycoproteins (GPs) is characteristic for apoptotic cells in vitro [Bilyy, R.O., Stoika, R.S., 2003. Lectinocytochemical detection of apoptotic murine leukemia L1210 cells. Cytometry 56A, 89-95]. It was independent of cell line or apoptosis-inducing agent, and can therefore be considered as a selective marker for identification and isolation of apoptotic cells [Bilyy, R.O., Antonyuk, V.O., Stoika, R.S., 2004. Cytochemical study of role of alpha-D-mannose- and beta-D-galactose-containing glycoproteins in apoptosis. J. Mol. Histol. 35, 829-838]. The main goals of the present study were: (1) to determine whether an increased expression of specific GPs also takes place after apoptosis induction in vivo; and (2) to identify additional characteristics of the membrane GP markers of the apoptotic cells. To reach these goals, we studied the expression of alpha-Man-rich membrane GPs in murine leukemia L1210 cells inoculated into abdominal cavities of mice which were then subjected to the action of apoptosis inducer doxorubicin. Another experimental model used in the present work was splenocytes obtained from mice treated with dexamethasone. Lectin-affinity chromatography and PAGE electrophoresis, or PAGE electrophoresis and lectinoblot analysis were applied for isolation of plasma membrane GPs (34 kDa, and high M(W) of approximately 600 and 800 kDa) whose expressions were increased during apoptosis. Triton X-114 treatment of cell membrane samples showed that the apoptotic cell-specific GPs were localized in the peripheral and integral compartments of plasma membrane. Apoptosis in vitro and in vivo was accompanied by an increased expression of the same GP, identified by MALDI-TOF MS analysis as the microtubule-actin cross-linking factor 1. Other GPs, whose expressions were also increased at apoptosis, were similarly identified as G-protein beta-subunit like (Acc# BAA06185.1) and dystonin isoform beta.

我们最近证实，富含α-D-甘露糖（Man）和β-D-半乳糖的质膜糖蛋白（GPs）表达增加是体外凋亡细胞的特征[Bilyy, R.O., Stoika, R.S., 2003. Lectinocytochemical detection of apoptotic murine leukemia L1210 cells. Cytometry 56A, 89 - 95]。它与细胞系或凋亡诱导剂无关，因此可被视为鉴定和分离凋亡细胞的选择性标志物[Bilyy, R.O., Antonyuk, V.O., Stoika, R.S., 2004. Cytochemical study of role of alpha-D-mannose- and beta-D-galactose-containing glycoproteins in apoptosis. J. Mol. Histol. 35, 829 - 838]。本研究的主要目标是：（1）确定体内诱导凋亡后特定GPs的表达是否也会增加；（2）确定凋亡细胞膜GP标志物的其他特征特征。为实现这些目标，我们研究了接种到小鼠腹腔中的鼠白血病L1210细胞中富含α-Man的膜GPs的表达，然后对其施加凋亡诱导剂阿霉素。本研究中使用的另一个实验模型是从用地塞米松处理的小鼠获得的脾细胞。采用凝集素亲和层析和PAGE电泳，或PAGE电泳和凝集素印迹分析来分离质膜GPs（34 kDa，以及高M（W）约为600和800 kDa），其表达在凋亡过程中增加。用Triton X - 114处理细胞膜样品表明，凋亡细胞特异性GPs定位于质膜的外周和整体部分。体外和体内凋亡均伴随着同一GP表达的增加，通过MALDI - TOF MS分析鉴定为微管 - 肌动蛋白交联因子1。其他在凋亡时表达也增加的GPs同样被鉴定为类G蛋白β亚基（Acc# BAA06185.1）和抗肌萎缩蛋白异构体β。