Pumplin D W, Fambrough D M
J Cell Biol. 1983 Oct;97(4):1214-25. doi: 10.1083/jcb.97.4.1214.
Immunofluorescence microscopy with a fluorescein-labeled monoclonal antibody was used to map the distribution of sodium- and potassium-ion stimulated ATPase [( Na,K]-ATPase) on the surface of tissue-cultured chick skeletal muscle. At this level of resolution it appeared that the (Na,K)-ATPase molecules were distributed nearly uniformly over the plasma membrane. These molecules could be cross-linked by use of the monoclonal antibody followed by a second antibody directed against the monoclonal antibody; the resulting fluorescent pattern was a set of small dots (patches) on the muscle surface. This pattern was stable over several hours, and there was little evidence of interiorization or of coalescence of the patches. Myotubes labeled with immunofluorescence were fixed in glutaraldehyde, cryoprotected with glycerin, then fractured and replicated by standard methods. Replicas of the immunofluorescence-labeled myotubes revealed clusters of intramembrane particles (IMP) only when the immunofluorescent images indicated a patching of the (Na,K)-ATPase molecules. Double antibody cross-linking of antigenic sites on myotubes with each of three other monoclonal antibodies to plasma membrane antigens likewise resulted in patched patterns of immunofluorescence, but in none of these cases were clusters of intramembrane particles found in freeze-fracture replicas. In each case it was shown that the (Na,K)-ATPase molecules were not patched. Other control experiments showed that patching of (Na,K)-ATPase molecules did not cause co-patching of one of the other plasma membrane proteins defined by a monoclonal antibody and did not cause detectable co-clustering of acetylcholine receptors. Detailed mapping showed that there was a one-to-one correspondence between immunofluorescent patches related to the (Na,K)-ATPase and clusters of IMP in a freeze-fracture replica of the same cell. We conclude that the intramembrane particles patched by double antibody cross-linkage of the (Na,K)-ATPase are caused by (Na,K)-ATPase molecules in the fracture plane. Quantification of the IMP indicated that the (Na,K)-ATPase-related particles account for up to 50% of particles evident in the replicas, or up to about 400 particles/micrometers2 of plasma membrane. Particles related to the (Na,K)-ATPase were similar to the average particle size and were as heterodisperse in size as the total population of IMP.(ABSTRACT TRUNCATED AT 400 WORDS)
使用荧光素标记的单克隆抗体进行免疫荧光显微镜检查,以绘制钠钾离子刺激的ATP酶[(Na,K)-ATP酶]在组织培养的鸡骨骼肌表面的分布。在这种分辨率水平下,(Na,K)-ATP酶分子似乎几乎均匀地分布在质膜上。通过使用单克隆抗体,然后使用针对该单克隆抗体的二抗,可以使这些分子交联;产生的荧光模式是肌肉表面上的一组小点(斑块)。这种模式在几个小时内是稳定的,几乎没有内化或斑块合并的迹象。用免疫荧光标记的肌管固定在戊二醛中,用甘油进行冷冻保护,然后通过标准方法进行断裂和复制。仅当免疫荧光图像显示(Na,K)-ATP酶分子出现斑块时,免疫荧光标记的肌管的复制品才显示出膜内颗粒(IMP)簇。用另外三种针对质膜抗原的单克隆抗体对肌管上的抗原位点进行双抗体交联,同样导致免疫荧光的斑块模式,但在这些情况下,冷冻断裂复制品中均未发现膜内颗粒簇。在每种情况下都表明,(Na,K)-ATP酶分子没有形成斑块。其他对照实验表明,(Na,K)-ATP酶分子的斑块化不会导致由单克隆抗体定义的其他质膜蛋白之一的共斑块化,也不会导致乙酰胆碱受体的可检测共聚集。详细的图谱显示,与(Na,K)-ATP酶相关的免疫荧光斑块与同一细胞的冷冻断裂复制品中的IMP簇之间存在一一对应关系。我们得出结论,通过(Na,K)-ATP酶的双抗体交联而形成斑块的膜内颗粒是由断裂平面中的(Na,K)-ATP酶分子引起的。对IMP的定量表明,与(Na,K)-ATP酶相关的颗粒占复制品中明显颗粒的50%,或高达约400个颗粒/微米²质膜。与(Na,K)-ATP酶相关的颗粒与平均颗粒大小相似,并且在大小上与IMP的总体一样具有多分散性。(摘要截断于400字)
