[Regulation of matrix-degrading enzymes in gynecologic cancer tissues and cells].

Nihon Sanka Fujinka Gakkai zasshi Pub Date : 1996-08-01
F Kikkawa
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引用次数: 0

Abstract

Introduction: Studies of tumor invasion and metastases have focused on the degradation of the basement membrane, which is predominantly made up of type IV collagen, laminin, and heparan sulfate proteoglycans. Matrix metalloproteinase-2 (MMP-2) and MMP-9, which can degrade type IV collagen, are implicated in cancer invasion and metastasis. Released and activated MMPs are controlled by specific tissue inhibitors of metalloproteinase (TIMP). In the present study, we have examined gelatinolytic and TIMP activity in the conditioned medium of human normal and cancer tissues by zymography and reverse zymography.

Materials and methods: 1) Tissues. Tissues were obtained at operation after informed consent was got from each patient. Sliced tissues were incubated in serum-free medium for 4 or 24 h at 37 degrees C. Human ovarian cancer cells (SAOV) were cultured for 24 h in serum-free medium containing conditioned medium of stromal tissues. After washing by PBS 3 times, SAOV cells were cultured for a further 24 h. 2) Zymography. Conditioned medium was subjected to SDS polyacrylamide gel containing 0.3 mg/ml of gelatin in zymography, and purified MMPs were added further in reverse zymography. After electrophoresis the gel was washed with Triton X-100, and incubated for 20 h at 37 degrees C in the reaction buffer. The gel was then stained with Coomassie brilliant blue. The gelatinase and TIMP activities were detected as unstained and stained bands, respectively. The photographs of the gels were scanned with a densitometer. 3) Other method. TIMP-1 levels of conditioned medium were assayed by ELISA kit. 4) Statistics. Statistical comparisons were made by Mann-Whiteny U test.

Results and discussion: We have examined the gelatinolytic activity in gynecologic normal and cancer tissues by zymography and reverse zymography. Ovarian, cervical, and endometrial cancer tissues demonstrated higher gelatinolytic activity than normal tissues. The major gelatinases were those with molecular weight of 92 and 72kD, which corresponded to MMP-9 and MMP-2, respectively. The ratio of MMP 9 to MMP-2 was significantly higher in 3 types of cancer tissues than in normal tissues. Reverse zymography demonstrated that TIMP-1 and TIMP-2 were present in all tissues, and the ratio of TIMP-1 to TIMP-2 was significantly higher in 3 types of cancer tissues than in normal tissues. These findings suggested that MMP-9 and TIMP-1 were more associated with cancer phenotype than other types of MMP and TIMP. The influence of human stromal tissues (peritoneum, myometrium, ovary) on the secretion of MMPs and TIMPs was examined by addition of these stromal tissues culture medium to human ovarian cancer cells (SAOV). All conditioned medium of stromal tissues could increase in both MMP-2, MMP-9, TIMP-1, and TIMP-2 activity in SAOV cells. Fraction (> 100kD) of conditioned medium of peritoneum could increase remarkably in MMP-9, and this increase could be inhibited by anti alpha 5 antibody, which is the most popular receptor of fibronectin. Furthermore, the addition of fibronectin to SAOV cells induced increase in the secretion of MMP-9. These results demonstrated that one of the factors included in conditioned medium of peritoneum was fibronectin. We found that interferon beta could suppressed the secretion of MMP-2 and invasion in choriocarcinoma cells. However, no effect of interferon beta was observed in SAOV cells. Several flavonoids were screened to have ability to suppress the secretion of MMPs. All trans retinoic acid (RA) could suppress the secretion of MMPs in SAOV cells in time and concentration dependent manners. Further, RA could inhibited the invasion of SAOV cells by invasion assay using boyden chamber coated with matrigel.

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[基质降解酶在妇科肿瘤组织和细胞中的调控作用]。
导言:肿瘤侵袭和转移的研究主要集中在基底膜的降解上,基底膜主要由IV型胶原蛋白、层粘连蛋白和硫酸肝素蛋白聚糖组成。基质金属蛋白酶-2 (MMP-2)和MMP-9可以降解IV型胶原,与癌症的侵袭和转移有关。金属蛋白酶的释放和活化是由金属蛋白酶(TIMP)的特异性组织抑制剂控制的。在本研究中,我们用酶谱法和反酶谱法检测了人正常组织和癌组织条件培养基中明胶溶解和TIMP活性。材料和方法:1)组织。在获得每位患者的知情同意后,于手术中获得组织。切片组织在37℃无血清培养基中培养4 h或24 h,人卵巢癌细胞(SAOV)在含基质组织条件培养基的无血清培养基中培养24 h。PBS洗涤3次后,SAOV细胞继续培养24小时。2)酶谱图。在条件培养基中加入含有0.3 mg/ml明胶的SDS聚丙烯酰胺凝胶进行酶谱分析,在反向酶谱分析中进一步加入纯化的MMPs。电泳后用Triton X-100洗涤凝胶,在37℃反应缓冲液中孵育20 h。然后用考马斯亮蓝染色。明胶酶和TIMP活性分别检测为未染色条带和染色条带。用密度计扫描凝胶的照片。3)其他方法。ELISA试剂盒检测条件培养基中TIMP-1水平。4)统计数据。统计学比较采用Mann-Whiteny U检验。结果和讨论:我们用酶谱法和反酶谱法检测了妇科正常组织和肿瘤组织的明胶溶解活性。卵巢癌、子宫颈和子宫内膜癌组织比正常组织显示出更高的明胶溶解活性。主要的明胶酶分子量为92和72kD,分别对应于MMP-9和MMP-2。3种癌组织中MMP- 9与MMP-2的比值均显著高于正常组织。反酶谱分析显示,TIMP-1和TIMP-2均存在于所有组织中,且3种癌组织中TIMP-1与TIMP-2的比值均显著高于正常组织。这些发现表明,MMP-9和TIMP-1比其他类型的MMP和TIMP更与癌症表型相关。通过将基质组织(腹膜、子宫肌层、卵巢)培养基加入人卵巢癌细胞(SAOV),观察基质组织对MMPs和TIMPs分泌的影响。基质组织条件培养基均可提高SAOV细胞的MMP-2、MMP-9、TIMP-1和TIMP-2活性。腹膜条件培养基中MMP-9含量(> 100kD)显著升高,且这种升高可被纤维连接蛋白最常见的受体抗α - 5抗体所抑制。此外,在SAOV细胞中加入纤维连接蛋白可诱导MMP-9分泌增加。这些结果表明,腹膜条件培养基中包含的因子之一是纤维连接蛋白。我们发现干扰素β可以抑制绒毛膜癌细胞中MMP-2的分泌和侵袭。然而,在SAOV细胞中未观察到干扰素β的作用。筛选了几种具有抑制MMPs分泌能力的类黄酮。所有反式维甲酸(RA)均能抑制SAOV细胞中MMPs的分泌,且呈时间和浓度依赖性。此外,在包膜基质的boyden室中进行的侵袭实验中,RA可以抑制SAOV细胞的侵袭。
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