Ca 2+ -Induced Conformational Change of Troponin C from the Japanese Pearl Oyster, Pinctada fucata

美国分子生物学期刊(英文) Pub Date : 2018-10-20 DOI:10.4236/ajmb.2018.84018

D. Funabara, D. Ishikawa, Yoshinori Urakawa, S. Kanoh

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引用次数: 3

Abstract

Troponin is a thin filament-associated regulator of vertebrate striated muscle contraction. Troponin changes its structure upon Ca2+ binding to troponin C, one of the subunits of troponin, allowing myosin to interact with actin. We recently elucidated the molecular characteristics of the Japanese pearl oyster Pinctada fucata troponin C (Pifuc-TnC), revealing the possibilities that Pifuc-TnC and vertebrate muscle TnC play dissimilar roles in muscle contraction. Pifuc-TnC has four EF-hand motifs, but, unlike vertebrate TnC, only one (site IV) was predicted to bind Ca2+. To confirm the number of Ca2+-binding sites in Pifuc-TnC and whether Ca2+ binding induces a conformational change, we purified the full-length protein and a variant, Pifuc-TnC-E142Q (that has a mutation in the predicted Ca2+-binding site of site IV), following their expression in laboratory E. coli. Isothermal titration calorimetry demonstrated Ca2+ binding to Pifuc-TnC, whereas Pifuc-TnC-E142Q was unable to bind Ca2+, confirming that site IV is the only Ca2+-binding site in Pifuc-TnC. Pifuc-TnC eluted in a later fraction from a gel filtration column in the presence of Ca2+ compared with the condition when Ca2+ was absent. In contrast, the elution profiles of Pifuc-TnC-E142Q were equivalent in both the presence and absence of Ca2+, suggesting that Ca2+ binding to Pifuc-TnC induces a conformational change that delays its elution from the column. UV-absorption spectral analysis revealed that binding of Ca2+ to Pifuc-TnC caused an increase in absorption at a wavelength of approximately 250 nm, possibly because phenylalanine residues had been exposed on the surface of the molecule as a result of a conformational change. Differential scanning calorimetric analyses of Pifuc-TnC showed aggregation in the presence of Ca2+ in accordance with an increase of temperature, but no aggregation was seen in the absence of Ca2+. In combination, these findings suggest that Ca2+ binding to site IV induces a conformational change in Pifuc-TnC.

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ca2 +诱导的日本珍珠贝肌钙蛋白C构象变化

肌钙蛋白是脊椎动物横纹肌收缩的细丝相关调节因子。肌钙蛋白在Ca2+与肌钙蛋白C（肌钙蛋白的亚基之一）结合时改变其结构，使肌球蛋白与肌动蛋白相互作用。我们最近阐明了日本珍珠牡蛎Pinctada fucata肌钙蛋白C（Pifuc TnC）的分子特征，揭示了Pifuc T nC和脊椎动物肌肉T nC在肌肉收缩中发挥不同作用的可能性。Pifuc-TnC有四个EF手基序，但与脊椎动物TnC不同，只有一个（位点IV）被预测与Ca2+结合。为了确认Pifuc-TnC中Ca2+结合位点的数量以及Ca2+结合是否诱导构象变化，我们纯化了全长蛋白和变异体Pifuc-TnC-E142Q（其在位点IV的预测Ca2+结合点中具有突变），随后它们在实验室大肠杆菌中表达。等温滴定量热法证明Ca2+与Pifuc-TnC结合，而Pifuc-TnC-E142Q不能结合Ca2+，证实了位点IV是Pifuc-TnC中唯一的Ca2+结合位点。与不存在Ca2+时的条件相比，在存在Ca2+的情况下，Pifuc-TnC在来自凝胶过滤柱的稍后级分中洗脱。相反，在存在和不存在Ca2+的情况下，Pifuc-TnC-E142Q的洗脱图谱是等效的，这表明Ca2+与Pifuc-TnC的结合诱导了构象变化，从而延迟了其从柱中的洗脱。UV吸收光谱分析显示，Ca2+与Pifuc-TnC的结合导致在大约250nm的波长下的吸收增加，这可能是因为苯丙氨酸残基由于构象变化而暴露在分子表面。Pifuc-TnC的差示扫描量热分析显示，随着温度的升高，在存在Ca2+的情况下发生聚集，但在不存在Ca2+时未观察到聚集。总之，这些发现表明Ca2+结合位点IV诱导Pifuc-TnC的构象变化。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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美国分子生物学期刊(英文)

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