首页> 外文期刊>Journal of nanoscience and nanotechnology >ATP Regeneration System Using E. coli ATP Synthase and Gloeobacter Rhodopsin and Its Stability
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ATP Regeneration System Using E. coli ATP Synthase and Gloeobacter Rhodopsin and Its Stability

机译:大肠杆菌ATP合酶和视紫红质球菌的ATP再生系统及其稳定性

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Great efforts in using non-photosynthetic bacteria as light-utilizing bacteria for producing biomaterials have been developed recently as increasing interest in renewable resources such as light energy. With respect to producing bio-materials industrially such as food ingredients and amino acids, huge amount of adenosine-5'-triphosphate (ATP) is required. In this work, we developed a bio-ATP-synthesis system using ATP synthase of Escherichia coli as a biocatalyst and a microbial rhodopsin which is from primitive cyanobacteria, Gloeobacter violaceus. Gloeobacter rhodopsin (GR) is a light-driven proton pump. Besides electro-chemical gradient produced by cellular respiration system, GR produces a proton gradient using light illumination which is used in additional driving force of synthesizing ATP by ATP synthase. Inverted membrane vesicle was prepared so that it could be incorporated with both of GR and ATP synthase and produced ATP in the exterior side of the vesicle in the presence of light. Since inverted membrane vesicle does not contain precursors for ATP, we added ADP and inorganic phosphate (P_i). Then, we measured the amounts of ATP produced by ATP synthase in the presence of light. As the average value of 6 samples, 4.79 × 10~(-2) μmole of ATP produced for 1 μg of GR per minute. Also, we measured again after 7 days and 65 days, respectively, in order to check the stability of the bio-ATP-synthesis system. Amount of ATP produced decayed double-exponentially and an expected value of half-life of the system was 1.5 days and 39.7 days. Our results demonstrate that ATP was regenerated successfully by using GR and ATP synthase. However, the stability of ATP synthase should be increased to use this system industrially in the near future.
机译:近来,随着人们对可再生资源如光能的兴趣日益增长,已在使用非光合细菌作为光利用细菌生产生物材料方面做出了巨大努力。对于工业生产生物材料,例如食品成分和氨基酸,需要大量的5'-三磷酸腺苷(ATP)。在这项工作中,我们开发了一种生物ATP合成系统,该系统利用大肠杆菌的ATP合酶作为生物催化剂和来自原始蓝细菌紫罗兰杆菌的微生物视紫红质。视紫红质球菌(GR)是光驱动的质子泵。除细胞呼吸系统产生的电化学梯度外,GR还使用光照明产生质子梯度,该质子梯度可用于由ATP合酶合成ATP的额外驱动力。制备倒膜囊泡,使其可以与GR和ATP合酶结合,并在有光的情况下在囊泡的外侧产生ATP。由于倒膜囊泡不包含ATP的前体,因此我们添加了ADP和无机磷酸盐(P_i)。然后,我们在有光的情况下测量了ATP合酶产生的ATP量。作为6个样品的平均值,每分钟1μgGR产生4.79×10〜(-2)μmolATP。此外,我们分别在7天和65天后再次进行测量,以检查bio-ATP合成系统的稳定性。产生的ATP量呈双指数衰减,系统的半衰期预期值为1.5天和39.7天。我们的结果表明,使用GR和ATP合酶可以成功地再生ATP。但是,应提高ATP合酶的稳定性,以在不久的将来工业上使用该系统。

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