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利用细胞壁锚定蛋白Pir在细胞表面构建的携带人α-1,3-岩藻糖基转移酶的酵母细胞。

Yeast cells harboring human alpha-1,3-fucosyltransferase at the cell surface engineered using Pir, a cell wall-anchored protein.

作者信息

Abe Hiroko, Ohba Mika, Shimma Yoh-ichi, Jigami Yoshifumi

机构信息

Research Center for Glycoscience (RCG), National Institute of Advanced Industrial Science and Technology (AIST), AIST Central 6, Tsukuba, Ibaraki 305-8566, Japan.

出版信息

FEMS Yeast Res. 2004 Jan;4(4-5):417-25. doi: 10.1016/S1567-1356(03)00193-4.

Abstract

Human alpha-1,3-fucosyltansferase (FucT) encoded by the FUT6 gene was displayed at the cell surface of yeast cells engineered using the yeast cell wall protein Pir1 or Pir2, and the FucT activity was detected at the surface of cells producing the Pir1-HA-FUT6 or Pir2-FLAG-FUT6 fusion proteins. To obtain higher activity, we engineered the host yeast cells in which endogenous PIR genes of the PIR1-4 gene family were disrupted. Among the disruptants, the pir1Delta pir2Delta pir3Delta strain with the PIR1-HA-FUT6 fusion gene showed the highest FucT activity, which was about three-fold higher than that of the wild-type strain. Furthermore, the co-expression of both the Pir1-HA-FUT6 and the Pir2-FLAG-FUT6 fusions showed an approximately 1.5-fold higher activity than that in the cell wall displaying Pir1-HA-FUT6 alone. The present method was thus effective for producing yeast cells that can easily synthesize various oligosaccharides, such as Le(x) and sLe(x), using Pir-glycosyltransferase fusions in combination with the deletion of endogenous PIR genes.

摘要

由FUT6基因编码的人α-1,3-岩藻糖基转移酶(FucT)展示在利用酵母细胞壁蛋白Pir1或Pir2构建的酵母细胞表面,并且在产生Pir1-HA-FUT6或Pir2-FLAG-FUT6融合蛋白的细胞表面检测到了FucT活性。为了获得更高的活性,我们构建了宿主酵母细胞,其中PIR1-4基因家族的内源性PIR基因被破坏。在这些破坏株中,带有PIR1-HA-FUT6融合基因的pir1Delta pir2Delta pir3Delta菌株显示出最高的FucT活性,比野生型菌株高出约三倍。此外,Pir1-HA-FUT6和Pir2-FLAG-FUT6融合蛋白的共表达显示出的活性比仅在细胞壁展示Pir1-HA-FUT6时高出约1.5倍。因此,本方法对于生产能够利用Pir-糖基转移酶融合蛋白并结合内源性PIR基因缺失轻松合成各种寡糖(如Le(x)和sLe(x))的酵母细胞是有效的。

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