Gierow J P, Lambert R W, Mircheff A K
Department of Cell & Neurobiology, University of Southern California, School of Medicine, Los Angeles 90033, USA.
Exp Eye Res. 1995 May;60(5):511-25. doi: 10.1016/s0014-4835(05)80066-1.
It is well known that lacrimal gland acinar cells retrieve secretory vesicle membrane constituents from their apical plasma membranes after stimulated exocytosis of secretory proteins. There have also been indications of a recycling traffic involving the basal-lateral plasma membranes. In an effort to document this traffic, determine how it is regulated, and discern whether it involves more than one intracellular compartment, we studied internalization of the fluid phase marker, Lucifer Yellow, and its relationship to protein release in acinar cells isolated from rabbit lacrimal glands. Loading of intracellular vesicles was apparent with fluoresence microscopy. Stimulation with carbachol increased both the rate of internalization and the intracellular volume equilibrating with extracellular fluid, suggesting the loading of two compartments. A carbachol concentration of 10 microM increased uptake by 80% during 20-min incubations at 37 degrees C. Increasing the carbachol concentration to 1 mM reduced the response by 50%, and it appeared to do so by decreasing the intracellular volume accessible to extracellular fluid, rather than the rate of endocytosis. Carbachol affected protein release differently, increasing it by 50% at 10 microM and 80% at 1 mM. Acceleration of endocytosis by 10 microM carbachol was transient, becoming negligible after 60 min. Vasoactive intestinal peptide (VIP) and isoproterenol increased internalization 35% and 25% respectively; neither reduced uptake at the highest concentrations tested; and only isoproterenol significantly affected protein secretion. Combinations of VIP and carbachol exerted synergistic effects on both fluid phase internalization and protein release. Steady-state uptake at 18 degrees C in the presence of 10 microM carbachol was equal to uptake at 37 degrees C in the absence of carbachol, suggesting a temperature block in the pathway to at least one endocytic compartment. Decreasing the temperature to 18 degrees C eliminated the inhibitory action of excessive carbachol, suggesting that the compartment whose loading was impaired by excessive carbachol was positioned distal to the temperature block. Carbachol accelerated release of marker from preloaded cells, indicating that it stimulated recycling between the plasma membranes and endocytic compartments. This effect was maximal at a concentration of 10 microM and unchanged with increasing concentrations. In accord with the hypothesis that traffic into and out of a certain compartment was particularly dependent on stimulation, a fraction of the marker taken up by optimally stimulated cells at 37 degrees C was retained unless carbachol or VIP was present in the efflux medium.(ABSTRACT TRUNCATED AT 400 WORDS)
众所周知,泪腺腺泡细胞在分泌蛋白受到刺激而发生胞吐作用后,会从其顶端质膜回收分泌囊泡膜成分。也有迹象表明存在涉及基底外侧质膜的循环运输。为了记录这种运输过程,确定其调控方式,并辨别它是否涉及不止一个细胞内区室,我们研究了液相标记物路西法黄在从兔泪腺分离的腺泡细胞中的内化及其与蛋白质释放的关系。通过荧光显微镜观察,细胞内囊泡的装载情况很明显。用卡巴胆碱刺激可增加内化速率以及与细胞外液达到平衡的细胞内体积,这表明有两个区室被装载。在37℃孵育20分钟期间,10微摩尔的卡巴胆碱浓度使摄取量增加了80%。将卡巴胆碱浓度增加到1毫摩尔会使反应降低50%,而且似乎是通过减少细胞外液可进入的细胞内体积,而非内吞作用速率来实现的。卡巴胆碱对蛋白质释放的影响不同,在10微摩尔时使其增加50%,在1毫摩尔时增加80%。10微摩尔的卡巴胆碱引起的内吞作用加速是短暂的,60分钟后就变得微不足道。血管活性肠肽(VIP)和异丙肾上腺素分别使内化增加35%和25%;在测试的最高浓度下两者都没有降低摄取量;并且只有异丙肾上腺素显著影响蛋白质分泌。VIP和卡巴胆碱的组合对液相内化和蛋白质释放都产生协同作用。在10微摩尔卡巴胆碱存在下于18℃的稳态摄取量与在37℃无卡巴胆碱时的摄取量相等,这表明在通往至少一个内吞区室的途径中存在温度阻滞。将温度降至18℃消除了过量卡巴胆碱的抑制作用,这表明被过量卡巴胆碱损害装载的区室位于温度阻滞的远端。卡巴胆碱加速了预装载细胞中标记物的释放,表明它刺激了质膜和内吞区室之间的循环。这种作用在10微摩尔浓度时最大,且随着浓度增加而不变。与进出某个区室的运输特别依赖刺激的假设一致,在37℃下经最佳刺激的细胞摄取的一部分标记物会被保留,除非在流出培养基中存在卡巴胆碱或VIP。(摘要截短至400字)
