Talarico Ernest F, Kennedy Brian G, Marfurt Carl F, Loeffler Karin U, Mangini Nancy J
Department of Anatomy & Cell Biology, Indiana University School of Medicine-Northwest, Gary, IN 46408-1197, USA.
Mol Vis. 2005 Mar 2;11:169-78.
Plasma membrane Ca2+-ATPases (PMCAs) are integral membrane proteins essential to the control of intracellular Ca2+ ([Ca2+]i) concentration. Four genes encode PMCA proteins termed PMCA1-PMCA4. Little is known about the expression of these isoforms in corneal epithelium (CE). The purpose of this investigation is to characterize the expression and distribution of PMCAs in human CE (hCE).
PMCA mRNA expression was examined by RT-PCR analysis of total RNA from native hCE using PMCA gene specific primers. PMCA isoform expression at the protein level in native hCE was examined by immunoblotting using isoform specific antibodies (Abs) and a panPMCA Ab that recognizes all PMCAs. Distribution of PMCAs in postmortem and surgical sections of hCE was determined by immunohistochemistry with the same Abs.
Immunoblot analysis with the panPMCA Ab yielded an intense band of approximately 135 kDa and several faintly staining bands above and below this major band. The isoform specific Abs labeled one or more bands that corresponded to bands detected with the panPMCA Ab. RT-PCR analysis of total RNA from hCE yielded PCR DNAs that were identified by sequencing as products of PMCA1, PMCA2, PMCA3, and PMCA4, thus confirming the immunoblot data. Immunohistochemistry demonstrated localization of PMCAs in all layers of hCE. PMCA4 was the predominant isoform, and was expressed along the plasma membrane of cells in all layers of CE, except with a notable absence along the basal cell membranes adjacent to the stroma. PMCA1 and PMCA2 were found mainly on basal and wing cells. In contrast to PMCA4, PMCA1 immunoreactivity (IR) was located on portions of basal cell plasma membranes adjacent to the stroma. PMCA2 IR was detected cytoplasmically within basal and wing cells in both central cornea and limbus. PMCA3 IR was located in basal cell nuclei in central cornea, but in a perinuclear location in the limbal, basal, and wing cells.
Human CE expresses multiple PMCA isoforms that are differentially expressed and localized among the layers and cells that comprise the CE. We propose that the differential expression of multiple PMCA isoforms affords CE the requisite flexibility to respond to the demands for Ca2+ regulation required during renewal and regeneration of its multiple cell types.
质膜钙ATP酶(PMCA)是控制细胞内钙离子([Ca2+]i)浓度所必需的整合膜蛋白。有四个基因编码称为PMCA1 - PMCA4的PMCA蛋白。关于这些异构体在角膜上皮(CE)中的表达知之甚少。本研究的目的是表征人角膜上皮(hCE)中PMCA的表达和分布。
使用PMCA基因特异性引物,通过对来自天然hCE的总RNA进行RT-PCR分析来检测PMCA mRNA表达。使用异构体特异性抗体(Abs)和识别所有PMCA的泛PMCA抗体,通过免疫印迹法检测天然hCE中蛋白质水平的PMCA异构体表达。使用相同的抗体通过免疫组织化学法确定PMCA在hCE的尸检和手术切片中的分布。
用泛PMCA抗体进行免疫印迹分析产生了一条约135 kDa的强条带以及该主要条带上下的几条淡染条带。异构体特异性抗体标记了一条或多条与用泛PMCA抗体检测到的条带相对应的条带。对hCE总RNA的RT-PCR分析产生了经测序鉴定为PMCA1、PMCA2、PMCA3和PMCA4产物的PCR DNA,从而证实了免疫印迹数据。免疫组织化学显示PMCA在hCE的所有层中均有定位。PMCA4是主要的异构体,在CE所有层的细胞的质膜上均有表达,但在与基质相邻的基底细胞膜上明显缺失。PMCA1和PMCA2主要在基底细胞和翼状细胞上发现。与PMCA4相反,PMCA1免疫反应性(IR)位于与基质相邻的基底细胞质膜部分。在中央角膜和角膜缘的基底细胞和翼状细胞的细胞质中检测到PMCA2 IR。PMCA3 IR位于中央角膜的基底细胞核中,但在角膜缘、基底和翼状细胞中位于核周位置。
人角膜上皮表达多种PMCA异构体,它们在构成角膜上皮的各层和细胞之间差异表达和定位。我们提出,多种PMCA异构体的差异表达为角膜上皮提供了必要的灵活性,以应对其多种细胞类型更新和再生过程中对钙离子调节的需求。
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