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Identification of a modori-inducing proteinase in the threadfin bream: Molecular cloning, tissue distribution and proteinase leakage from viscera during ice storage

机译:在冰蓄冷中鉴定透射灌注中的蛋白酶诱导蛋白酶:冰储存过程中的分子克隆,组织分布和蛋白酶泄漏

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摘要

Previously we purified and characterized a sarcoplasmic serine proteinase (SSP) from the belly muscle of the threadfin bream as a modori-inducing proteinase. In our attempt to clarify the structure and physiological functions of SSP, we successfully cloned the full-length cDNA of SSP (ORF 726 bp). The deduced amino acid sequence of SSP (241 residues) was highly homologous to fish trypsinogen. The distribution of SSP mRNA and the proteinase activity in the tissue indicated that SSP was mainly synthesized and existed in the digestive system under physiological conditions. After ice storage of the threadfin bream without gutting, a high SSP activity was detected only in the belly muscle because of SSP leaked from the viscera. Therefore, it is desirable to use edible proteinase inhibitor to inactivate the leaked SSP during production of surimi-based products or to take effective measures to prevent the proteinase leakage during post-harvest storage.
机译:以前我们纯化并表征了从雷丝鲷的腹部肌肉作为模卤诱导蛋白酶的腹肌丝氨酸蛋白酶(SSP)。我们试图澄清SSP的结构和生理功能,我们成功地克隆了SSP的全长cDNA(ORF 726 BP)。 SSP(241个残基)的推导的氨基酸序列与鱼胰蛋白酶原具有高度同源。组织中SSP mRNA的分布和组织中的蛋白酶活性表明SSP主要合成并存在于生理条件下的消化系统中。在没有咀嚼的透射丝鲷的冰蓄冷后,由于SSP从内脏泄漏,仅在腹部肌肉中检测到高SSP活性。因此,希望在生产基于Surimi的产品期间使用食用蛋白酶抑制剂将泄漏的SSP灭活,或采取有效措施,以防止收获后储存期间蛋白酶泄漏。

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