蛋清溶菌酶分离纯化实验的改进

蛋白质分离纯化技术是生化及分子生物学实验技术的重要组成部分,在本科实验教学中占有重要地位。为了探索合适的实验方法和实验条件,优化本科实验教学中的溶菌酶分离纯化实验,以获得更好的纯化结果和教学效果,该文使用离子交换层析、硫铵沉淀、分子筛层析等方法成功地从蛋清中纯化出高纯度的溶菌酶,用SDS-聚丙烯酰胺凝胶电泳方法鉴定了样品纯度,并用溶壁微球菌做为底物测定了纯化酶的活力及比活力。结果显示,使用改进后的方法能够得到较高纯度和比活力的溶菌酶,整个实验重复性好、易于操作,适合作为本科教学实验项目。

对于本科实验教学中蛋清溶菌酶分离纯化实验的改进

蛋白质的分离纯化技术是生物化学的重要基础,在本科实验教学中占有重要地位。本科教学实验中的溶菌酶分离纯化实验是有助于学生了解并掌握蛋白质的分离纯化技术的经典实验,但在实际操作中有所欠缺。为了获得更好地实验结果与教学效果,本文对实验做了一定改进,利用离子交换层析、硫酸铵沉淀、分子筛层析等方法从鸡蛋清中获取溶菌酶,用SDS-PAGE电泳进行鉴定,并对溶菌酶进行了结晶、定性和定量上测定溶菌酶活力,尽量涉及了蛋白质实验的多个领域,且重复性好,易于学生操作,可更加有利于学生对蛋白质性质的理解乃至对之前所学实验的理解,培养学生的独立科研能力。

Simultaneous Cell Disruption and Aqueous Two-Phase Extraction for Isolation of Intracellular Recombinant Proteins

A new technique was developed for the integrated processing of cell disruption and aqueous two-phase extraction in a high-speed bead mill to separate intracellular proteins from microbial cells. The process was named as simultaneous cell disruption and aqueous two-phase extraction (SDATE). Advantages, such as high cell disruption efficiency, biochemical activities preservation of proteins, cell debris elimination, and prelimiary purification of the target protein were being claimed. When this technique was employed for isolating recombinant Tumor Necrosis Factor (TNF) from E. coli, overall protein concentration and TNF activity were found to have been increased. More than 95% of TNF was partitioned into the top phase and all cell debris were in the bottom phase. The partition coefficient was greater than 3 and the TNF purification factor was greater than 6. It is shown that less separation steps were being utilized in the new technique, meaning a reduction in separation time and less process extractors required.