Rebres R A, McKeown-Longo P J, Vincent P A, Cho E, Saba T M
Department of Physiology and Cell Biology, Albany Medical College, New York 12208, USA.
Am J Physiol. 1995 Dec;269(6 Pt 1):G902-12. doi: 10.1152/ajpgi.1995.269.6.G902.
The incorporation of plasma fibronectin (pFn) into the extracellular matrix (ECM) is believed to influence tissue integrity, wound repair, and vascular permeability. In vitro, matrix assembly of Fn requires the binding of soluble Fn to cell-associated matrix assembly sites. Alkylation of human pFn (HFn) with N-ethylmaleimide (NEM) prevents the initial binding of Fn to matrix assembly sites as well as its in vitro incorporation into the ECM as reflected by detergent-insoluble 125I-labeled Fn (pool II Fn). We determined the kinetics of Fn matrix incorporation in tissue and whether NEM treatment of rat pFn (NEM-RFn) would limit its in vivo incorporation into ECM by analysis of pool I [deoxycholate (DOC) soluble] and pool II (DOC insoluble) 125I-Fn in tissues after its intravenous injection into rats. After intravenous injection, tissue incorporation of normal rat 125I-pFn was especially intense in liver and spleen, in agreement with the large amount of endogenous Fn detected in the matrices of these organs. Tissue deposition of plasma-derived 125I-RFn in liver and spleen peaked by 4 h, with significant (P < 0.01) loss over 24 h, indicating turnover of matrix Fn. Tissue localization of normal 125I-RFn in liver, lung, spleen, heart, and intestine was greater (P < 0.05) than 125I-NEM-RFn at 4 h. Normal HFn, but not NEM-HFn, was incorporated into tissues and colocalized with endogenous Fn in the matrix. To identify the cells mediating the intense incorporation of pFn into liver ECM, we compared matrix assembly of 125I-HFn by cultured fibroblasts, hepatocytes, and hepatic Kupffer cells. With fibroblasts, 125I-HFn in pool I reached steady state by 3 h, whereas 125I-HFn in pool II exceeded that in pool I by 6 h and continued to increase over 24 h. With hepatocytes, pool I 125I-HFn reached steady state by 1 h, and a progressive increase (P < 0.05) of 125I-HFn in pool II was observed over 24 h. Kupffer cells were not able to incorporate significant amounts of 125I-HFn into matrix. NEM-HFn displayed limited incorporation into ECM by both fibroblast and hepatocyte cultures. These novel observations suggest that the interaction of soluble pFn with matrix assembly sites is necessary to its in vivo incorporation into the ECM.
血浆纤连蛋白(pFn)掺入细胞外基质(ECM)被认为会影响组织完整性、伤口修复和血管通透性。在体外,Fn的基质组装需要可溶性Fn与细胞相关的基质组装位点结合。用人pFn(HFn)与N - 乙基马来酰亚胺(NEM)进行烷基化反应可阻止Fn与基质组装位点的初始结合,以及其在体外掺入ECM,这可通过去污剂不溶性的125I标记的Fn(池II Fn)反映出来。我们通过分析静脉注射到大鼠体内后组织中池I [脱氧胆酸盐(DOC)可溶性]和池II(DOC不溶性)125I - Fn,确定了Fn在组织中基质掺入的动力学,以及NEM处理大鼠pFn(NEM - RFn)是否会限制其在体内掺入ECM。静脉注射后,正常大鼠125I - pFn在肝脏和脾脏中的组织掺入特别强烈,这与在这些器官的基质中检测到的大量内源性Fn一致。血浆来源的125I - RFn在肝脏和脾脏中的组织沉积在4小时达到峰值,在24小时内有显著(P < 0.01)损失,表明基质Fn有周转。在4小时时,正常125I - RFn在肝脏、肺、脾脏、心脏和肠道中的组织定位比125I - NEM - RFn更高(P < 0.05)。正常HFn而非NEM - HFn被掺入组织并与基质中的内源性Fn共定位。为了确定介导pFn强烈掺入肝脏ECM的细胞,我们比较了培养的成纤维细胞、肝细胞和肝库普弗细胞对125I - HFn的基质组装情况。对于成纤维细胞,池I中的125I - HFn在3小时达到稳态,而池II中的125I - HFn在6小时超过池I中的,并在24小时内持续增加。对于肝细胞,池I中的125I - HFn在1小时达到稳态,并且在24小时内观察到池II中的125I - HFn有逐渐增加(P < 0.05)。库普弗细胞不能将大量的125I - HFn掺入基质。NEM - HFn在成纤维细胞和肝细胞培养物中显示出有限的掺入ECM的能力。这些新的观察结果表明,可溶性pFn与基质组装位点的相互作用对其在体内掺入ECM是必要的。
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