Dong J T, Rinker-Schaeffer C W, Ichikawa T, Barrett J C, Isaacs J T
Johns Hopkins Oncology Center, Johns Hopkins University of School of Medicine, Baltimore, Maryland, USA.
World J Urol. 1996;14(3):182-9. doi: 10.1007/BF00186898.
Prostate cancer is one of the most commonly diagnosed cancers and is a major cause of cancer death in men. Although the majority of the diagnosed prostate cancers will remain localized and never produce clinical symptoms during the lifetime of the host, a subset of these cancers will progress to a more malignant state requiring therapeutic intervention. Acquisition of metastatic ability by prostatic cancer cells is the most lethal aspect of prostatic cancer progression. Once this has occurred, definitive therapy is required before the initially localized metastatic cells escape from the prostate. At present, metastatic prostate cancer is incurable. Therefore, there is an urgent need to develop molecular markers that can be used to predict the metastatic potential of prostate cancers. Using somatic cell hybridization, we have demonstrated that acquisition of metastatic ability requires both the loss of metastasis-suppressor function(s) and the activation of oncogenes. In further studies using micro-cell-mediated chromosomal transfer, we located genes on human chromosome, 8, 10cen-q23, 11p11.2-13, and 17pter-q23, which, when introduced into rat prostatic cancer cells, are capable of suppressing their metastatic ability without affecting their tumorigenicity or growth rate in vivo. Initially we focused upon the human chromosome 11p11.2-13 region to clone metastasis-suppressor gene(s) positionally. One such gene, termed KAI-1, encodes a membrane glycoprotein. KAI-1 has been mapped to the p11.2 region of human chromosome 11 by fluorescence in-situ hybridization analysis. Expression of KAI-1 has been detected in all normal human tissues thus far tested, including prostate tissue. When introduced into rat metastatic prostatic cancer cells, KAI-1 significantly suppressed the metastasis without affecting the tumor growth rate. KAI-1 expression is high in human normal prostate and benign prostatic hyperplasia but is dramatically lower in cancer cell lines derived from metastatic prostate tumors.
前列腺癌是最常被诊断出的癌症之一,也是男性癌症死亡的主要原因。尽管大多数被诊断出的前列腺癌会保持局部状态,在宿主的一生中都不会产生临床症状,但其中一部分癌症会发展为更恶性的状态,需要进行治疗干预。前列腺癌细胞获得转移能力是前列腺癌进展中最致命的方面。一旦发生这种情况,在最初局部的转移细胞从前列腺逃逸之前就需要进行确定性治疗。目前,转移性前列腺癌无法治愈。因此,迫切需要开发可用于预测前列腺癌转移潜能的分子标志物。通过体细胞杂交,我们已经证明获得转移能力既需要转移抑制功能的丧失,也需要癌基因的激活。在使用微细胞介导的染色体转移的进一步研究中,我们在人类染色体8、10cen-q23、11p11.2-13和17pter-q23上定位了一些基因,当将这些基因导入大鼠前列腺癌细胞时,它们能够抑制其转移能力,而不影响其在体内的致瘤性或生长速率。最初我们聚焦于人类染色体11p11.2-13区域,以定位克隆转移抑制基因。其中一个这样的基因,称为KAI-1,编码一种膜糖蛋白。通过荧光原位杂交分析,KAI-1已被定位到人类染色体11的p11.2区域。到目前为止,在所有测试过的正常人体组织中都检测到了KAI-1的表达,包括前列腺组织。当将KAI-1导入大鼠转移性前列腺癌细胞时,它能显著抑制转移,而不影响肿瘤生长速率。KAI-1在人类正常前列腺和良性前列腺增生中表达较高,但在源自转移性前列腺肿瘤的癌细胞系中显著降低。
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