GOLD/FAB IMMUNE ELECTRON-MICROSCOPY LOCALIZATION OF TROPONIN-H AND TROPONIN-T IN LETHOCERUS FLIGHT-MUSCLE

被引:40
作者
REEDY, MC [1 ]
REEDY, MK [1 ]
LEONARD, KR [1 ]
BULLARD, B [1 ]
机构
[1] EUROPEAN MOLEC BIOL LAB,W-6900 HEIDELBERG,GERMANY
关键词
MUSCLE; ULTRASTRUCTURE; TROPONIN; THIN FILAMENTS; IMMUNO EM;
D O I
10.1006/jmbi.1994.1350
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The position of the large troponin complex relative to myosin crossbridges in Lethocerus flight muscle (IFM) has been probed by electron microscopy (EM) using monoclonal antibodies against troponin T (TnT) and troponin H (TnH), a heavy troponin component found in several insect muscles. Infiltration of gold-tagged and plain Fab fragments into glycerinated IFM before fixation established in non-overlap fibers that the beads every 38·7 nm along thin filaments are troponin. Original and optically filtered EM images from 25 nm longitudinal and 15 nm cross-sections of partially overlapped fibers suggests that epitopes on both TnT and TnH are very close to the rear crossbridge of the rigor double chevron. When Fab was infiltrated into relaxed fibers and ATP was subsequently removed, the resulting rigor crossbridge lattice was disrupted by antibody labeling of the troponin. The results confirm that the lattice of rigor crossbridges and troponin are congruent and suggest that crossbridges may interact with troponin in IFM, possibly serving as a partial basis for the stretch activation characteristic of this muscle. © 1994 Academic Press Limited.
引用
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页码:52 / 67
页数:16
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