α2-巨球蛋白可抑制转化生长因子-β诱导的人肝肌成纤维细胞胶原蛋白合成。

Transforming growth factor-beta-induced collagen synthesis by human liver myofibroblasts is inhibited by alpha2-macroglobulin.

作者信息

Tiggelman A M, Linthorst C, Boers W, Brand H S, Chamuleau R A

机构信息

Academic Medical Center, University of Amsterdam, J van Gool Laboratory for Experimental Internal Medicine, The Netherlands.

出版信息

J Hepatol. 1997 Jun;26(6):1220-8. doi: 10.1016/s0168-8278(97)80455-2.

DOI:10.1016/s0168-8278(97)80455-2

PMID:9210607

Abstract

BACKGROUND

Transforming growth factor-beta (TGFbeta) plays a central role in the stimulation of matrix production during liver fibrosis. The action of TGFbeta in different systems has been shown to be influenced by alpha2-macroglobulin (alpha2M), a serum protein with strong protease-scavenging and cytokine-binding properties.

AIMS

In the present study, alpha2M derived from normal human plasma has been tested for its ability to modulate the TGFbeta-induced collagen production by human liver fat-storing cells (FSC), which had transformed into alpha-smooth muscle actin-expressing myofibroblasts in culture.

METHODS

Alpha2M has been tested after activation with methylamine (alpha2M-Me), an in vitro equivalent of protease activated alpha2M. The binding of 125I-TGFbeta1 to activated forms of alpha2M was demonstrated by rate electrophoresis. Collagen synthesis was examined in human liver myofibroblast cultures obtained from three different human livers by incorporation of 3H-proline into TCA-precipitable, specific collagenase degradable proteins. Uptake of alpha2M was studied by means of immunofluorescence.

RESULTS

TGFbeta (1 ng/ml) significantly stimulated collagen synthesis of controls in the absence of TGFbeta. Alpha2M-Me reduced this TGFbeta-induced collagen synthesis dose-dependently, reaching significant inhibition from 10 microg/ml alpha2M-Me onward. Upon addition of 100 microg/ml alpha2M-Me the effect of TGFbeta was reduced by 60% to 128+/-31% (mean+/-SD) of control values in the absence of TGFbeta. Human liver myofibroblasts endocytosed alpha2M-Me added to the cultures as detected by immunofluorescence. Accordingly, reduction of TGFbeta-activity by alpha2M-Me may be explained by receptor-mediated clearance of alpha2M-TGFbeta complexes by the cells.

CONCLUSIONS

TGFbeta-induced collagen formation by human liver myofibroblasts obtained from three different livers is reduced in vitro by activated alpha2M. From these results, we hypothesize that alpha2M may have an antifibrogenic effect in vivo by interference with TGFbeta-induced matrix synthesis during liver fibrosis.

摘要

背景

转化生长因子-β（TGFβ）在肝纤维化过程中刺激基质产生方面发挥核心作用。TGFβ在不同系统中的作用已被证明受α2-巨球蛋白（α2M）影响，α2M是一种具有强大蛋白酶清除和细胞因子结合特性的血清蛋白。

目的

在本研究中，已对源自正常人血浆的α2M调节人肝贮脂细胞（FSC）中TGFβ诱导的胶原蛋白产生的能力进行了测试，这些细胞在培养中已转化为表达α-平滑肌肌动蛋白的肌成纤维细胞。

方法

用甲胺（α2M-Me）激活后的α2M进行了测试，甲胺是蛋白酶激活的α2M的体外等效物。通过速率电泳证明了125I-TGFβ1与激活形式的α2M的结合。通过将3H-脯氨酸掺入三氯乙酸沉淀的、可被特异性胶原酶降解的蛋白质中，在从三个不同人肝脏获得的人肝肌成纤维细胞培养物中检测胶原蛋白合成。通过免疫荧光研究α2M的摄取。

结果

在不存在TGFβ的情况下，TGFβ（1 ng/ml）显著刺激了对照的胶原蛋白合成。α2M-Me剂量依赖性地降低了这种TGFβ诱导的胶原蛋白合成，从10 μg/ml α2M-Me起达到显著抑制。加入100 μg/ml α2M-Me后，TGFβ的作用在不存在TGFβ时降低至对照值的60%，即128±31%（平均值±标准差）。通过免疫荧光检测发现，人肝肌成纤维细胞内吞了添加到培养物中的α2M-Me。因此，α2M-Me降低TGFβ活性可能是由于细胞通过受体介导清除α2M-TGFβ复合物所致。