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Thy-1 在血管內皮細胞遷移所扮演的角色 The roles of Thy-1 in the migration of endothelial cells

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Thy-1 在血管內皮細胞遷移所扮演的角色

The roles of Thy-1 in the migration of endothelial cells

 本篇論文的主旨是在探討 Thy-1 在血管增生過程中所扮演的角色。在過去的文獻中指出,血管增生 現象在許多生理及病理現象中都扮演相當重要的角色。例如當腫瘤形成時,為了從活體中得到大量 養分以及進行物質交換,腫瘤會釋放出血管增生因子與周邊血管上的接受器結合,促使血管內皮細 胞向腫瘤的方向移動,並且逐漸形成新生之血管。而針對控制癌症的血管增生現象,成為目前治療 癌症的很重要的方向。由於內皮細胞在產生發炎反應、癌症、或是懷孕時期,新增生的血管會有 T hy-1 大量表現,本實驗室利用人類臍帶靜脈內皮細胞 (human umbilical vein endothelial cell, HUVEC) 來探討 Thy-1 對血管增生的影響。我們首先利用基因轉殖的方法將 Thy-1 送入內皮細胞中,使其過 度表現後,再利用西方點墨法以及反轉錄 - 聚合酶連鎖反應實驗證實在蛋白質或是在 RNA 層級都 會有過度表現的現象發生。而在 Thy-1 過度表現時,我們進行了細胞增生及遷移實驗,並且發現到 Thy-1 過度表現之後,內皮細胞的增生並未受影響,而遷移之內皮細胞數則有顯著的減少現象。因 為細胞貼附能力也會影響到細胞的遷移現象,接著我們進行了細胞貼附及存活實驗,結果發現到,

Thy-1 的過量表現對於細胞貼附及細胞的存活率並沒有明顯的影響,所以推測 Thy-1 可能不是藉由 改變細胞貼附的能力來調控細胞遷移。此外,在血管構造形成的實驗中也發現,若 Thy-1 過度表現 時,內皮細胞形成管狀的能力會明顯的受到抑制。接著我們針對細胞遷移相關蛋白質進行西方點墨 法實驗,發現到 Rho family 之 Rho A 、 Rho B 、 Rho C 等細胞遷移相關蛋白質表現都受到了明顯 的抑制。 Rho 蛋白質會因為其在細胞內之表現聚集位置不同而產生不同的效應,所以我們接著進 行質膜分離的實驗,我們將細胞質與細胞膜分開萃取,並且進行西方點墨法的實驗,分別偵測其分 布位置上的差異,我們發現到分布於細胞質的 Rho A ,其表現量在 Thy-1 過量表現的組別中,有明 顯上升的情況。此外,我們藉由 Rho AV14 以及 ROCK 抑制劑的作用,利用細胞遷移分析實驗證實

, Thy-1 過度表現所造成的內皮細胞遷移及管腔形成的抑制現象,主要是藉由 Rho-mediated pathwa y 所造成。綜合以上實驗結果我們可以發現, Thy-1 的過度表現會抑制 Rho 蛋白質的表現,並且藉 由 Rho-mediated pathway 達到抑制細胞遷移的現象,也藉由未知的分子路徑抑制血管內皮細胞之血 管構造形成。

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 It has been recognized that angiogenesis is required in many physiological and pathological co

nditions. For instance, in the development of tumor, in order to get more nutrients, tumor cells

promote vessel formation through the expression of angiogenic molecules in the microenviron

ment. The understanding that the growth of tumors depends on the acquisition of a blood supp

ly has led to the development of new therapies strategy for cancer based on inhibition of angio

genesis. Previously, our laboratory has demonstrated that Thy-1 molecule was expressed in mi

crovascular endothelial cells during angiogenesis and served as a marker for angiogenesis. Th

e aim of this thesis study is to examine the roles of Thy-1 molecule during angiogenesis. To ga

in this purpose, we over-expressed Thy-1 protein by transfection of Thy-1 cDNA into HUVE

C. Our data demonstrated that over-expression of Thy-1 did not affect the proliferation of end

othelial cells, but inhibited the HUVEC migration, capillary-like tube formation, and down-re

gulated the Rho protein. Over-expression of Thy-1 did not affect the adhesion and viability of

HUVEC, suggesting that Thy-1-induced inhibition of endothelial cell migration was not throu

gh altering the cell adhesion or the occurrence cell death. Moreover, we found that over-expre

ssion of RhoA V14 dramatically reversed the Thy-1-induced inhibition of cell migration and t

ube formation. However, pretreatment of the cells with ROCK inhibitor abolished the preventi

on effect of RhoA V14 on Thy-1-induced migration inhibition and tube formation. Taken toge

ther, these data suggest that Rho family might play an important role in the Thy-1-induced mi

gration inhibition of HUVEC.

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