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首页> 外文期刊>Journal of Biotechnology >Expression and purification of bioactive soluble murine stem cell factor from recombinant Escherichia coli using thioredoxin as fusion partner
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Expression and purification of bioactive soluble murine stem cell factor from recombinant Escherichia coli using thioredoxin as fusion partner

机译:以硫氧还蛋白为融合伴侣从重组大肠杆菌中表达和纯化生物活性可溶性鼠干细胞因子

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摘要

Stem cell factor (SCF) known as the c-kit ligand, plays important roles in spermatogenesis, melanogenesis and early stages of hematopoiesis. As for the latter, SCF is essential for growth and expansion of hematopoietic stem and progenitor cells. We herein describe the production of recombinant murine SCF from Escherichia coli as soluble thioredoxin-fusion protein. The formation of insoluble and inactive inclusion bodies, usually observed when SCF is expressed in E. coli, was almost entirely prevented. After purification based on membrane adsorber technology, the fusion protein was subsequently cleaved by TEV protease in order to release mature mSCF. Following dialysis and a final purification step, the target protein was isolated in high purity. Bioactivity of mSCF was proven by different tests (MTT analogous assay, long-term proliferation assay) applying a human megakaryocytic cell line. Furthermore, the biological activity of the uncleaved fusion protein was tested as well. We observed a significant activity, even though it was less than the activity displayed by the purified mSCF. In summary, avoiding inclusion body formation we present an efficient production procedure for mSCF, one of the most important stem cell cytokines
机译:被称为c-kit配体的干细胞因子(SCF)在精子生成,黑色素生成和造血的早期阶段起着重要作用。至于后者,SCF对于造血干细胞和祖细胞的生长和扩展至关重要。我们在此描述了作为可溶性硫氧还蛋白融合蛋白从大肠杆菌生产重组鼠SCF。当在大肠杆菌中表达SCF时通常观察到的不溶性和非活性包涵体的形成几乎被完全阻止。基于膜吸附技术纯化后,融合蛋白随后被TEV蛋白酶裂解,以释放成熟的mSCF。透析和最终纯化步骤后,高纯度分离出目标蛋白。通过使用人巨核细胞系的不同测试(MTT类似测定,长期增殖测定)证明了mSCF的生物活性。此外,还测试了未切割的融合蛋白的生物学活性。我们观察到了显着的活性,即使该活性低于纯化的mSCF所显示的活性。总之,为避免包涵体形成,我们提出了一种有效的生产程序,用于生产最重要的干细胞细胞因子之一的mSCF。

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