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从赤子爱胜蚓中提取的强效纤溶酶的纯化及蛋白质组学分析

Purification and proteomic analysis of potent fibrinolytic enzymes extracted from Lumbricus rubellus.

作者信息

Stephani Laurentia, Rahayu Puji, Retnoningrum Debbie, Suhartono Maggy Thenawidjaja, Rachmawati Heni, Tjandrawinata Raymond R

机构信息

Biopharmaceutical Technology Division, Research Innovation and Invention, Dexa Laboratories of Biomolecular Sciences, PT Dexa Medica, Kawasan Industri Jababeka II, Industri Selatan V Block PP No. 7, Cikarang, 17550, Indonesia.

Research Group of Pharmaceutics, School of Pharmacy, Bandung Institute of Technology, Bandung, Indonesia.

出版信息

Proteome Sci. 2023 May 8;21(1):8. doi: 10.1186/s12953-023-00206-9.

Abstract

BACKGROUND

Lumbrokinase derived from earthworms, Lumbricus rubellus is known to have fibrinolytic enzymes that have potential as therapeutic drugs due to its ability to dissolve fibrin. The current study is aimed to purify the Lumbrokinase from L. rubellus and identify its protein component.

METHODS

Water extract of local earthworm Lumbricus rubellus revealed several proteins. Therefore, to identify its protein component, purification through HiPrep DEAE fast flow and proteomic analysis were conducted prior to identifications. A combination of two-dimension gel electrophoresis (2DE) and electrospray ionization mass spectrometry analysis was used to identify the purified fractions.

RESULTS

The purified fractions contain five protein bands, namely F25-1, F25-2, F85-1, F85-2, and F85-3, which displayed strong fibrinogenolytic activity. F25 fractions showed fibrinogenolytic activity of 974.85 U/mg, while F85 fractions showed higher activity of 1,484.11 U/mg. Fractions F85-1, F85-2, and F85-3 showed molecular weights of 42.6 kDa, 27.03 kDa, and 14 kDa, respectively and were identified as Lumbrokinase iso-enzymes.

CONCLUSION

This preliminary study indicates that the F25 and F85 fractions are similar to published fibrinolytic protease-1 and lumbrokinase, respectively, in terms of their amino acid sequence.

摘要

背景

源自赤子爱胜蚓的蚓激酶已知含有纤维蛋白溶解酶,因其溶解纤维蛋白的能力而具有作为治疗药物的潜力。当前研究旨在从赤子爱胜蚓中纯化蚓激酶并鉴定其蛋白质成分。

方法

当地赤子爱胜蚓的水提取物显示出几种蛋白质。因此,为了鉴定其蛋白质成分,在鉴定之前先通过HiPrep DEAE快速流动法进行纯化并进行蛋白质组学分析。采用二维凝胶电泳(2DE)和电喷雾电离质谱分析相结合的方法来鉴定纯化后的组分。

结果

纯化后的组分含有五条蛋白带,即F25 - 1、F25 - 2、F85 - 1、F85 - 2和F85 - 3,它们表现出很强的纤维蛋白原溶解活性。F25组分的纤维蛋白原溶解活性为974.85 U/mg,而F85组分表现出更高的活性,为1484.11 U/mg。F85 - 1、F85 - 2和F85 - 3组分的分子量分别为42.6 kDa、27.03 kDa和14 kDa,并被鉴定为蚓激酶同工酶。

结论

这项初步研究表明,F25和F85组分在氨基酸序列方面分别与已发表的纤维蛋白溶解蛋白酶-1和蚓激酶相似。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dc72/10165752/e150b72f32c9/12953_2023_206_Fig1_HTML.jpg

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