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The structure–function relationship of MSI7, a matrix protein from pearl oyster <italic>Pinctada fucata</italic>
Author(s) -
Qiaoli Feng,
Zi Fang,
Zhenguang Yan,
Rui Xing,
Liping Xie,
Rongqing Zhang
Publication year - 2009
Publication title -
acta biochimica et biophysica sinica
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.771
H-Index - 57
eISSN - 1745-7270
pISSN - 1672-9145
DOI - 10.1093/abbs/gmp086
Subject(s) - pinctada fucata , aragonite , crystallization , calcite , nucleation , crystallography , protein subunit , chemistry , biophysics , recombinant dna , biology , biochemistry , mineralogy , pearl , pearl oyster , gene , philosophy , theology , organic chemistry
We previously identified a matrix protein, MSI7, from pearl oyster Pinctada fucata. According to the structural analysis, the DGD site in the N-terminal of MSI7 is crucial for its role in the shell formation. In this study, we expressed a series of recombinant MSI7 proteins, including the wild-type and several mutants directed at the DGD site, using an Escherichia coli expression system to reveal the structure-function relationship of MSI7. Furthermore, in vitro crystallization, crystallization speed assay, and circular dichroism spectrometry were carried out. Results indicated that wild-type MSI7 could induce the nucleation of aragonite and inhibit the crystallization of calcite. However, none of the mutants could induce the nucleation of aragonite, but all of them could inhibit the crystallization of calcite to some extent. And all the proteins accelerated the crystallization process. Taken together, the results indicated that MSI7 could contribute to aragonite crystallization by inducing the nucleation of aragonite and inhibiting the crystallization of calcite, which agrees with our prediction about its role in the nacreous layer formation of the shell. The DGD site was critical for the induction of the nucleation of aragonite.

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