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组织型纤溶酶原激活剂与小鼠小脑颗粒神经元的结合

Tissue plasminogen activator binding to mouse cerebellar granule neurons.

作者信息

Verrall S, Seeds N W

机构信息

Department of Biochemistry/Biophysics/Genetics, University of Colorado Medical School, Denver 80262.

出版信息

J Neurosci Res. 1988 Oct-Dec;21(2-4):420-5. doi: 10.1002/jnr.490210233.

Abstract

Cultures of dissociated neonatal mouse cerebellar cells secrete primarily tissue plasminogen activator (tPA) and to a lesser extent urokinase plasminogen activator (uPA) into the culture medium. Fibrin overlays have localized plasminogen activator to granule neurons in these cultures; furthermore, this granule cell plasminogen activator activity is blocked by an antibody to tPA. Developmental studies indicate that maximal levels of soluble plasminogen activator in the culture medium preceed the peak of fibrinolytic activity by these cultures, suggesting that secreted PA may bind back to the surface of these granule neurons. Here we show that granule cell-associated tPA can be displaced by a brief pH shock. However, incubation of these fibrinolytically inactive cultures with exogenously added mouse tPA leads to a specific binding of active tPA to granule neurons as visualized by subsequent fibrin overlay. In similar studies mouse uPA, human uPa, and human tPA fail to show fibrinolytic activity associated with the cerebellar culture, whereas mouse tPA fails to bind to cerebellar glial cell cultures. These findings suggest that granule neurons possess binding sites for tPA on their surface, where this protease can retain its functional activity and may play an important role in cell migration or other cell activities.

摘要

新生小鼠小脑细胞解离培养物主要向培养基中分泌组织型纤溶酶原激活物(tPA),尿激酶型纤溶酶原激活物(uPA)的分泌量较少。纤维蛋白覆盖法已将纤溶酶原激活物定位到这些培养物中的颗粒神经元;此外,这种颗粒细胞纤溶酶原激活物活性被抗tPA抗体阻断。发育研究表明,培养基中可溶性纤溶酶原激活物的最高水平先于这些培养物的纤溶活性峰值出现,这表明分泌的PA可能会重新结合到这些颗粒神经元的表面。在此我们表明,短暂的pH冲击可使颗粒细胞相关的tPA移位。然而,用外源添加的小鼠tPA孵育这些无纤溶活性的培养物,会导致活性tPA与颗粒神经元特异性结合,后续的纤维蛋白覆盖法可观察到这一现象。在类似研究中,小鼠uPA、人uPA和人tPA均未显示与小脑培养物相关的纤溶活性,而小鼠tPA未与小脑胶质细胞培养物结合。这些发现表明,颗粒神经元表面存在tPA的结合位点,该蛋白酶可在这些位点保持其功能活性,并可能在细胞迁移或其他细胞活动中发挥重要作用。

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