The role of the sulfhydryl groups of tropomyosin and troponin in the calcium control of actomyosin contractility.

Methods for preparing troponin and tropomyosin from ethanol-extracted muscle are presented. Examination of these proteins by disc electrophoresis indicated that the troponin preparation is homogeneous. If precautions were taken to assure that the -SH groups of tropomyosin were not permitted to oxidize during preparation or electrophoresis, tropomyosin appeared to be nearly homogeneous. Traces of troponin, however, appeared in all samplds. Neither troponin nor tropomyosin was found to make actomyosin superprecipitation sensitive to the removal of Ca+f. Combined, they were effective. A moderately wide range of troponin to tropomyosin ratios (between 1: 1 and 3 : 1) were found to provide optimal sensitization of actomyosin. At a troponin to tropomyosin ratio of 1.3 : 1, 35 pg of this protein mixture inhibited by 85% 200 pg of actomyosin. The ability of troponin to collaborate with tropomyosin in the sensitization of actomyosin was lost to varying degrees if the troponin --SH groups were allowed to react with p-chloromercuribenzoate or N-ethyhnaleimide or if the -SH groups were not protected during preparation. In contrast, the function of tropomyosin was found not to correlate with the state of its -SH groups. Troponin was found to be a potent calcium-binding substance, possessing 24 pmoles of high affinity calcium-binding sites per g. The high affinity site had an apparent affinity constant of approximately 2.4 X 10” M-‘. It is hypothesized that the binding of calcium to this site inactivates troponin and that this is the mechanism whereby calcium activates myofibrillar contraction. It is concluded that tropomyosin does not possess a similar class of calcium-binding sites. The affinity of troponin for calcium was unaltered by reaction of its -SH groups. The number of high affinity calciumbinding sites was, however, doubled to approximately 40