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Biosequestration of carbon dioxide using a silicified carbonic anhydrase catalyst

机译:使用硅化碳酸酐酶催化剂生物固存二氧化碳

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摘要

Using recombinant DNA technology, we constructed a dual fusion gene expression plasmid, pRCAH-30, encoding carbonic anhydrase (CA) from the cyanobacterium Synechocystis sp. PCC6803, an R5 peptide sequence, and an affinity (His)6 tag, to allow the simultaneous purification and immobilization of the encoded fusion enzyme, termed RCAH. The expressed fusion protein was approximately 30 kDa, and could be rapidly purified using affinity resins. To enhance enzyme activity, the R5 peptide facilitated immobilization by means of silicification with tetramethoxysilane; the aggregated particles were approximately 300 nm in diameter. Activity tests revealed that the enzyme functioned optimally between pH 7.0 and 7.5; maximum stability was achieved between 25 and 45°C, at pH 6.0 ∼ 8.0. Activity of the fusion enzyme persisted, even after encapsulation by biomimetic silicification. In fact, silicone embedding stabilized the enzyme structure, thereby increasing its stability and reusability rate under different environmental conditions. In addition, the silicified enzyme reduced waste CO2 gas from 800 to 42 ppm, resulting in a gas capture rate of 94.7% after conversion. Thus, the construct developed in this study can be effectively utilized for the sequestration of industrial waste CO2 gas.
机译:使用重组DNA技术,我们构建了双融合基因表达质粒pRCAH-30,编码来自蓝藻集胞藻(Synechocystcystis sp。)的碳酸酐酶(CA)。 PCC6803,一个R5肽序列和一个亲和(His)6标签,以允许同时纯化和固定被编码为RCAH的编码融合酶。表达的融合蛋白约为30 kDa,可以使用亲和树脂快速纯化。为了增强酶活性,R5肽通过用四甲氧基硅烷硅化来促进固定化。聚集的颗粒的直径约为300nm。活性测试表明,该酶在pH 7.0和7.5之间具有最佳功能。在pH 6.0〜8.0的25至45°C之间达到最大稳定性。甚至在通过仿生硅化进行包封之后,融合酶的活性仍然存在。实际上,有机硅包埋可稳定酶的结构,从而提高其在不同环境条件下的稳定性和可重复使用率。另外,硅化酶将废气中的CO2气体从800 ppm减少到42 ppm,转化后的气体捕获率为94.7%。因此,在这项研究中开发的构造可以有效地用于隔离工业废气中的CO2气体。

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