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首页> 外文期刊>Molecular and Cellular Biochemistry: An International Journal for Chemical Biology >Rapid, simple and sensitive microassay for skeletal muscle homogenates in the functional assessment of the Ca-release channel of sarcoplasmic reticulum: Application to diagnosis of susceptibility to malignant hyperthermia
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Rapid, simple and sensitive microassay for skeletal muscle homogenates in the functional assessment of the Ca-release channel of sarcoplasmic reticulum: Application to diagnosis of susceptibility to malignant hyperthermia

机译:快速,简单,灵敏的骨骼肌匀浆微量测定在肌浆网钙释放通道功能评估中的应用:在恶性高热敏感性诊断中的应用

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摘要

A microassay is demonstrated for functional characterization of the Ca2+-release channel (CRC) of sarcoplasmic reticulum (SR) of skeletal muscle using swine with susceptibility to malignant hyperthermia (MH). Diluted muscle homogenates, indo-1 and ratiometric dual-emission spectrofluorometry are used to monitor Ca2+-lowering activity in real-time in the presence and absence of ryanodine at exposures that open and close the CRC. Reactions are initiated with 50 μM CaCl2 to raise ionized Ca2+ concentration near 1 μM and MgATP to activate the Ca2+-ATPase pump. Oxalate is included to precipitate Ca2+ within the SR. The assay requires less than 30 mg muscle, which may be cryopreserved, and is completed within 20 min of thawing the tissue. Maximum SR Ca2+-ATPase pumping and CRC activities, degree of CRC activation, and Ca2+-buffering capacity can be determined. Using this assay we studied muscle from MH-susceptible swine and demonstrated that whereas maximal Ca2+-ATPase pumping and CRC activities are normal, the CRC activity after addition of a bolus of Ca2+ is 50% greater in heterozygotes and 100% greater in homozygotes for the MH mutation. Hypersensitivity to CRC agonists, such as caffeine, and an associated hyposensitivity to CRC antagonists such as Mg2+ is also demonstrated. Genotypes for the MH mutation site can be discriminated from each other by determining Ca2+-lowering activities and the effect of ryanodine on them.
机译:证明了使用猪对恶性高热(MH)敏感的骨骼肌肌质网(SR)的Ca2 +释放通道(CRC)的功能表征的微量测定。稀释的肌肉匀浆,indo-1和比例双发射光谱法用于在打开和关闭CRC的暴露条件下,实时监测存在或不存在ryanodine的Ca2 +降低活性。用50μMCaCl2引发反应,使离子化的Ca2 +浓度升高至1μM附近,并用MgATP激活Ca2 + -ATPase泵。包含草酸盐以在SR中沉淀Ca2 +。该测定需要少于30 mg的肌肉,可将其冷冻保存,并在解冻组织后20分钟内完成。可以确定最大SR Ca2 + -ATPase抽运和CRC活性,CRC活化程度以及Ca2 +缓冲能力。使用这种测定方法,我们研究了MH敏感猪的肌肉,并证明尽管最大的Ca2 + -ATPase泵送和CRC活性是正常的,但添加Ca2 +推注后,杂合子的CRC活性高50%,纯合子的CRC活性高100%。 MH突变。还显示了对CRC激动剂(例如咖啡因)的超敏性以及对CRC拮抗剂(例如Mg2 +)的相关超敏性。 MH突变位点的基因型可以通过确定降低Ca2 +的活性以及雷诺丹对它们的作用来区分。

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