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视黄酸对转移性大鼠乳腺腺癌细胞IV型胶原酶解及穿过重组基底膜侵袭的抑制作用。

Inhibition by retinoic acid of type IV collagenolysis and invasion through reconstituted basement membrane by metastatic rat mammary adenocarcinoma cells.

作者信息

Nakajima M, Lotan D, Baig M M, Carralero R M, Wood W R, Hendrix M J, Lotan R

机构信息

Department of Tumor Biology, University of Texas, M.D. Anderson Cancer Center, Houston 77030.

出版信息

Cancer Res. 1989 Apr 1;49(7):1698-706.

PMID:2538232
Abstract

The activity of type IV collagenase, which enables tumor cells to degrade collagen type IV found in the subendothelial basement membrane, has been correlated with the metastatic potential in several tumor types, including the rat 13762NF mammary adenocarcinoma cell line and its clones. In this study, we examined whether all-trans-retinoic acid (all-trans-RA) and other retinoids, which exhibit antitumor activity in vitro and in vivo, affect the collagenolytic activity of metastatic rat 13762NF mammary adenocarcinoma cells. Cells of the highly metastatic lung-colonizing clone MTF7.T35.3, derived from the 13762NF cell line, were treated for 3 days with 0.1, 1, or 10 microM all-trans-RA, harvested, and seeded on [3H]proline-labeled extracellular matrix deposited by cultured rat lung endothelial cells or on a film of purified [3H]proline-labeled type IV collagen. The amount of radioactivity released into the medium during the subsequent 24 to 72 h was measured, and it was found that all-trans-RA treatment inhibited degradation of extracellular matrix and type IV collagen by 50 to 60%. This effect was observed whether the cells had been treated with all-trans-RA in serum-free medium or in medium supplemented with heat-inactivated or acid-treated fetal bovine serum. The growth of the cells was not inhibited under these conditions, except after treatment with 10 microM all-trans-RA in serum-free medium. The reduction in collagenolytic activity was observed in viable cells as well as in conditioned medium. A 24-h exposure of cells to all-trans-RA was sufficient to cause a 30% decrease in the collagenolytic activity, and this inhibitory effect was reversible. The direct addition of all-trans-RA to conditioned medium had no effect on secreted collagenase activity. The apparent molecular weights of the collagenolytic enzymes were determined by electrophoresis of cell extracts and concentrated conditioned medium in type IV collagen-embedded polyacrylamide gels followed by renaturation and activation of the enzymes within the gels. Two major type IV collagenolytic metalloproteinases exhibiting molecular weights of 64,000 and 88,000, respectively, were detected by this method. These two enzymes were also found to have specificity for gelatin. The Mr 64,000 enzyme could be extracted from viable cells (presumably from the cell membrane) by 2% 1-butanol. Treatment with all-trans-RA decreased the level of these enzymes in the cellular, cell membrane, and conditioned medium compartments.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

IV型胶原酶能够使肿瘤细胞降解在内皮下基底膜中发现的IV型胶原,其活性已与包括大鼠13762NF乳腺腺癌细胞系及其克隆在内的几种肿瘤类型的转移潜能相关。在本研究中,我们检测了在体外和体内均具有抗肿瘤活性的全反式维甲酸(all-trans-RA)和其他类维生素A是否会影响转移性大鼠13762NF乳腺腺癌细胞的胶原溶解活性。用0.1、1或10 microM全反式维甲酸处理源自13762NF细胞系的高转移性肺定植克隆MTF7.T35.3的细胞3天,收获细胞,并接种于由培养的大鼠肺内皮细胞沉积的[3H]脯氨酸标记的细胞外基质上,或接种于纯化的[3H]脯氨酸标记的IV型胶原膜上。测量随后24至72小时内释放到培养基中的放射性量,发现全反式维甲酸处理可使细胞外基质和IV型胶原的降解抑制50%至60%。无论细胞是在无血清培养基中还是在补充有热灭活或酸处理胎牛血清的培养基中用全反式维甲酸处理,均观察到这种效果。在这些条件下,细胞生长未受抑制,但在无血清培养基中用10 microM全反式维甲酸处理后除外。在活细胞以及条件培养基中均观察到胶原溶解活性降低。细胞暴露于全反式维甲酸24小时足以使胶原溶解活性降低30%,且这种抑制作用是可逆的。将全反式维甲酸直接添加到条件培养基中对分泌的胶原酶活性没有影响。通过在IV型胶原包埋的聚丙烯酰胺凝胶中对细胞提取物和浓缩的条件培养基进行电泳,然后在凝胶内使酶复性并激活,来测定胶原溶解酶的表观分子量。通过该方法检测到两种主要的IV型胶原溶解金属蛋白酶,其分子量分别为64,000和88,000。还发现这两种酶对明胶具有特异性。Mr 64,000的酶可以用2%正丁醇从活细胞(可能从细胞膜)中提取。用全反式维甲酸处理可降低细胞、细胞膜和条件培养基组分中这些酶的水平。(摘要截短至400字)

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