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利用CPMV-HT瞬时表达系统在本氏烟草中表达活性重组人胃脂肪酶。

Expression of active recombinant human gastric lipase in Nicotiana benthamiana using the CPMV-HT transient expression system.

作者信息

Vardakou Maria, Sainsbury Frank, Rigby Neil, Mulholland Francis, Lomonossoff George P

机构信息

Institute of Food Research, Norwich Research Park, Norwich NR4 7UA, UK.

Department of Biological Chemistry, John Innes Centre, Norwich Research Park, Norwich NR4 7UH, UK.

出版信息

Protein Expr Purif. 2012 Jan;81(1):69-74. doi: 10.1016/j.pep.2011.09.005. Epub 2011 Sep 17.

DOI:10.1016/j.pep.2011.09.005
PMID:21945702
Abstract

Recombinant human gastric lipase (hGL) was transiently expressed in Nicotiana benthamiana leaves using the CPMV-HT expression system. Expression levels of up to 0.5mg recombinant hGL per gram of infiltrated leaf tissue were obtained. Proteins expressed from two hGL constructs, wild type (wt-hGL) and with a Histidine tag at its C terminal (hGL-His), were purified from leaf tissue using Immobilized Lectin Affinity chromatography and Immobilized Metal Affinity chromatography. Both variants were glycosylated, enzymatically active, and had an apparent molecular weight similar to native hGL (approx. 50kDa). The recombinant hGLs were stable under acidic conditions and in the presence of gastric pepsin. Moreover, as found with the naturally occurring enzyme, the activity of recombinant hGL on the short chain lipid, tributyrin, was higher than on long chain Intralipid 30% emulsion. The maximum specific activity measured on tributyrin was 310 U/mg of protein and the maximum yield was 193 U/g of infiltrated leaf tissue. These results show that transient expression in plants can be used to produce active hGL that could be efficiently purified using established techniques. The approach provides a means of generating large quantities of hGL that could be of use for a number of applications both in vitro and in vivo.

摘要

使用CPMV-HT表达系统在本氏烟草叶片中瞬时表达重组人胃脂肪酶(hGL)。每克浸润叶组织获得高达0.5mg重组hGL的表达水平。从叶组织中使用固定化凝集素亲和色谱法和固定化金属亲和色谱法纯化了从两种hGL构建体表达的蛋白质,即野生型(wt-hGL)及其C末端带有组氨酸标签的(hGL-His)。两种变体均被糖基化,具有酶活性,并且表观分子量与天然hGL相似(约50kDa)。重组hGL在酸性条件下和存在胃蛋白酶的情况下是稳定的。此外,正如天然存在的酶一样,重组hGL对短链脂质三丁酸甘油酯的活性高于对长链英脱利匹特30%乳剂的活性。在三丁酸甘油酯上测得的最大比活性为310U/mg蛋白质,最大产量为193U/g浸润叶组织。这些结果表明,在植物中瞬时表达可用于生产活性hGL,其可使用既定技术有效纯化。该方法提供了一种产生大量hGL的手段,可用于许多体外和体内应用。

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