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表面展示猴金属硫蛋白 α 串联重复序列和 EGFP 融合蛋白在铜绿假单胞菌 X4 上,用于生物吸附和检测镉。

Surface display of monkey metallothionein α tandem repeats and EGFP fusion protein on Pseudomonas putida X4 for biosorption and detection of cadmium.

机构信息

State Key Laboratory of Agricultural Microbiology, Huazhong Agricultural University, Wuhan 430070, China.

出版信息

Appl Microbiol Biotechnol. 2012 Sep;95(6):1605-13. doi: 10.1007/s00253-011-3768-3. Epub 2011 Dec 29.

Abstract

Monkey metallothionein α domain tandem repeats (4mMTα), which exhibit high cadmium affinity, have been displayed for the first time on the surface of a bacterium using ice nucleation protein N-domain (inaXN) protein from the Xanthomonas campestris pv (ACCC-10049) as an anchoring motif. The shuttle vector pIME, which codes for INAXN-4mMTα-EGFP fusion, was constructed and used to target 4mMTα and EGFP on the surface of Pseudomonas putida X4 (CCTCC-209319). The surface location of the INAXN-4mMTα-EGFP fusion was further verified by western blot analysis and immunofluorescence microscopy. The growth of X4 showed resistance to cadmium presence. The presence of surface-exposed 4mMTα on the engineered strains was four times higher than that of the wild-type X4. The Cd²⁺ accumulation by X4/pIME was not only four times greater than that of the original host bacterial cells but was also remarkably unaffected by the presence of Cu²⁺ and Zn²⁺. Moreover, the surface-engineered strains could effectively bind Cd²⁺ under a wide range of pH levels, from 4 to 7. P. putida X4/pIME with surface-expressed 4mMTα-EGFP had twice the cadmium binding capacity as well as 1.4 times the fluorescence as the cytoplasmic 4mMTa-EGFP. These results suggest that P. putida X4 expressing 4mMTα-EGFP with the INAXN anchor motif on the surface would be a useful tool for the remediation and biodetection of environmental cadmium contaminants.

摘要

首次使用来自黄单胞菌(Xanthomonas campestris pv)的冰核蛋白 N 结构域(inaXN)蛋白作为锚定基序,在细菌表面展示了具有高镉亲和力的猴金属硫蛋白α 结构域串联重复序列(4mMTα)。构建了编码 INAXN-4mMTα-EGFP 融合蛋白的穿梭载体 pIME,并将其用于将 4mMTα 和 EGFP 靶向到假单胞菌 X4(CCTCC-209319)的表面。通过 Western blot 分析和免疫荧光显微镜进一步验证了 INAXN-4mMTα-EGFP 融合蛋白的表面定位。X4 的生长表现出对镉存在的抗性。工程菌株表面暴露的 4mMTα 含量比野生型 X4 高四倍。X4/pIME 积累的 Cd²⁺不仅比原始宿主细菌细胞高四倍,而且不受 Cu²⁺和 Zn²⁺的存在显著影响。此外,表面工程菌株在 pH 值范围从 4 到 7 的广泛范围内可以有效结合 Cd²⁺。表面表达 4mMTα-EGFP 的 P. putida X4/pIME 的镉结合能力是细胞质 4mMTa-EGFP 的两倍,荧光强度是细胞质 4mMTa-EGFP 的 1.4 倍。这些结果表明,表达表面展示的 4mMTα-EGFP 的 P. putida X4 与 INAXN 锚定基序结合,将成为修复和生物检测环境镉污染物的有用工具。

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