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CN111172068B - Construction method and application of periplasmic photosensitized whole-cell hybrid system - Google Patents

Construction method and application of periplasmic photosensitized whole-cell hybrid system Download PDF

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CN111172068B
CN111172068B CN202010022433.2A CN202010022433A CN111172068B CN 111172068 B CN111172068 B CN 111172068B CN 202010022433 A CN202010022433 A CN 202010022433A CN 111172068 B CN111172068 B CN 111172068B
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施伟东
罗必富
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Abstract

本发明属于生物‑无机复合材料技术领域,涉及一种细胞周质光敏化的全细胞杂合体系的构筑方法,包括:选择能够进行细胞周质表达生物酶的细菌细胞接种到对应培养基中,有氧条件下进行活化后,将菌液和培养液按1:100比例转移至新培养瓶中,待细菌浓度达到0.4~0.6后,进行厌氧处理使其在细胞周质表达生物酶;然后,在厌氧条件下加入半导体纳米光敏化剂,置于30℃的恒温摇床中进行细胞杂合;最后对溶液进行离心、洗涤,再将细胞周质光敏化的全细胞杂合体系重悬到新的反应缓冲溶液中。本发明通过具有广谱吸收范围的半导体纳米粒子与在细胞周质中表达生物酶的细胞来构筑,用以实现太阳能‑化学能的高效转化,在环境、能源等领域有良好应用前景。

Figure 202010022433

The invention belongs to the technical field of biological-inorganic composite materials, and relates to a method for constructing a periplasmic photosensitized whole-cell hybrid system, comprising: selecting bacterial cells capable of expressing biological enzymes in the periplasm and inoculating them into corresponding culture medium, After activation under aerobic conditions, transfer the bacteria solution and culture solution to a new culture bottle at a ratio of 1:100. After the bacterial concentration reaches 0.4-0.6, perform anaerobic treatment to express biological enzymes in the periplasm; then , add semiconductor nano-photosensitizer under anaerobic conditions, place in a constant temperature shaker at 30°C for cell hybridization; finally, centrifuge and wash the solution, and then resuspend the periplasmic photosensitized whole-cell hybrid system into a new reaction buffer solution. The invention is constructed by semiconductor nanoparticles with broad-spectrum absorption range and cells expressing biological enzymes in the periplasm to realize efficient conversion of solar energy to chemical energy, and has good application prospects in the fields of environment and energy.

Figure 202010022433

Description

细胞周质光敏化的全细胞杂合体系的构筑方法及其应用Construction method and application of periplasmic photosensitized whole-cell hybrid system

技术领域technical field

本发明属于生物-无机复合材料技术领域,涉及细胞杂合,尤其涉及一种细胞周质光敏化的全细胞杂合体系的构筑方法及其应用。The invention belongs to the technical field of biological-inorganic composite materials, and relates to cell hybridization, in particular to a method for constructing a periplasmic photosensitized whole-cell hybrid system and its application.

背景技术Background technique

半导体光催化纳米材料因其良好的光捕获能力、稳定性以及催化活性,在解决能源危机和环境问题等方面的潜在应用价值而日益受到人们的关注。然而,半导体光催化纳米材料本身催化活性位点少,催化反应缓慢,制约了其进一步应用。为了弥补这个不足,近年来,由于生物酶的专一性和高效性,生物酶逐渐应用于太阳能-化学能的转化。通过半导体催化材料与生物酶结合,生物酶作为高效的催化活性位点,半导体材料作为光敏化剂,进而实现太阳能-化学能的高效转化。虽然这种无机-生物酶杂合体系具有较高的催化性能,但是生物酶本身纯化步骤复杂,产率低以及对氧气比较敏感,导致其应用亦受到限制。Semiconductor photocatalytic nanomaterials have attracted increasing attention because of their good light-harvesting ability, stability and catalytic activity, and their potential application value in solving energy crisis and environmental problems. However, semiconductor photocatalytic nanomaterials have few catalytic active sites and slow catalytic reactions, which restrict their further applications. In order to make up for this deficiency, in recent years, due to the specificity and high efficiency of biological enzymes, biological enzymes have been gradually applied to the conversion of solar energy to chemical energy. Through the combination of semiconductor catalytic materials and biological enzymes, biological enzymes serve as efficient catalytic active sites, and semiconductor materials serve as photosensitizers, thereby realizing efficient conversion of solar energy to chemical energy. Although this inorganic-biological enzyme hybrid system has high catalytic performance, the purification steps of the biological enzyme itself are complicated, the yield is low, and it is relatively sensitive to oxygen, which limits its application.

近年来,利用可以表达生物酶的全细胞替代生物酶为构筑新型无机-生物杂合体系提供了新的思路。相比于纯的生物酶,细胞具有容易获得、稳定以及自我修复的优点。基于此,Honda等人利用TiO2光催化剂与E.coli首次构筑了无机-生物全细胞杂合体系(Honda, Y.; Hagiwara, H.; Ida, S.; Ishihara, T. Angew. Chem. Int. Edit. 2016,55, 8045-8048),实现高效的分解水产氢性能。TiO2作为光敏化剂,光激发后的电子通过电子中介体甲基紫精的跨膜过程传递到细胞的生物酶,在生物酶上实现太阳能转化;其不足之处在于电子的跨膜传递过程缓慢,且需要消耗额外的能量,导致电子的转移效率不高。为了克服这个问题,杨培东等人提出了一种胞内光敏作用的全细胞体系(Zhang, H.; Liu,H.; Tian, Z.; Lu, D.; Yu, Y.; Cestellos-Blanco, S.; Sakimoto, K. K.; Yang, P.Nat. Nanotechnol. 2018, 13, 900-905),他们把金纳米簇生长到细胞内,从而使光敏化剂(Au纳米簇)的光激发和电子的转移过程均在细胞质中进行,有效地提升了电子转移效率。必须指出的是,该体系中由于细胞质中成分复杂,光的传输会受到干扰,光敏化剂的光吸收因此也会受到影响。In recent years, the use of whole cells that can express biological enzymes to replace biological enzymes has provided a new idea for the construction of new inorganic-biological hybrid systems. Compared with pure biological enzymes, cells have the advantages of easy acquisition, stability and self-healing. Based on this, Honda et al. used TiO 2 photocatalyst and E.coli to construct the inorganic-biological whole-cell hybrid system for the first time (Honda, Y.; Hagiwara, H.; Ida, S.; Ishihara, T. Angew. Chem. Int. Edit. 2016,55, 8045-8048), to achieve efficient water splitting performance for hydrogen production. TiO 2 is used as a photosensitizer, and the electrons after photoexcitation are transferred to the biological enzymes of the cells through the transmembrane process of the electron mediator methyl viologen, and the solar energy conversion is realized on the biological enzymes; the disadvantage lies in the transmembrane transfer process of electrons It is slow and consumes extra energy, resulting in inefficient transfer of electrons. To overcome this problem, Yang et al. proposed a whole-cell system for intracellular photosensitization (Zhang, H.; Liu, H.; Tian, Z.; Lu, D.; Yu, Y.; Cestellos-Blanco, S.; Sakimoto, KK; Yang, P. Nat. Nanotechnol. 2018, 13, 900-905), who grew gold nanoclusters into cells so that photoexcitation of photosensitizers (Au nanoclusters) and electronic The transfer process is carried out in the cytoplasm, which effectively improves the electron transfer efficiency. It must be pointed out that due to the complex components in the cytoplasm in this system, the transmission of light will be disturbed, and the light absorption of the photosensitizer will also be affected.

在细菌细胞中,细胞外膜与内膜之间存在着细胞周质。与细胞质相比,它与外膜的距离更近,可以减少光传输中的干扰,更利于光敏化剂的光吸收。此外,其具有较小的空间可以使生物酶有较高的局域浓度,增加了光敏化剂与生物酶的接触,加快催化反应的发生。发明人构建了一种细胞周质光敏化的全细胞杂合体系。通过调控,将生物兼容性良好的光催化纳米材料(如TiO2, NaTaO3, KTaO3, Bi3TaO7, WO3, Bi2O3, BiVO4, CdS, CuIn2S4/ZnSQDs, g-C3N4等)生长到能在细胞周质表达生物酶的细胞(如Shewanella oneidensisDesulfovibrio gigas, Desulfovibrio vulgaris, Desulfovibrio desulfuricans,Desulfovibrio baculatus等)中;同时实现有效的光吸收和电子转移,实现高效的太阳能-化学能转化。In bacterial cells, the periplasm exists between the outer and inner membranes of the cell. Compared with the cytoplasm, it is closer to the outer membrane, which can reduce interference in light transmission and is more conducive to the light absorption of photosensitizers. In addition, it has a smaller space, which can make the biological enzyme have a higher local concentration, increase the contact between the photosensitizer and the biological enzyme, and accelerate the occurrence of the catalytic reaction. The inventors constructed a whole-cell hybrid system with periplasmic photosensitization. By regulation, biocompatible photocatalytic nanomaterials (such as TiO 2 , NaTaO 3 , KTaO 3 , Bi 3 TaO 7 , WO 3 , Bi 2 O 3 , BiVO 4 , CdS, CuIn 2 S 4 /ZnSQDs, gC 3 N 4 , etc.) to grow into cells that can express biological enzymes in the periplasm (such as Shewanella oneidensis , Desulfovibrio gigas , Desulfovibrio vulgaris , Desulfovibrio desulfuricans , Desulfovibrio baculatus , etc.); simultaneously achieve effective light absorption and electron transfer, and achieve efficient Solar-to-chemical energy conversion.

迄今为止,尚未发现有细胞周质光敏化的全细胞杂合体系构筑的报道。So far, there has been no report on the construction of a periplasmic photosensitized whole-cell hybrid system.

发明内容Contents of the invention

本发明目的是提供一种普适性的细胞周质光敏化的全细胞杂合体系的构筑方法,用以实现太阳能-化学能的高效转化。The purpose of the present invention is to provide a universal method for constructing a periplasmic photosensitized whole-cell hybrid system to realize efficient conversion of solar energy to chemical energy.

技术方案Technical solutions

一种细胞周质光敏化的全细胞杂合体系的构筑方法,包括如下步骤:A method for constructing a periplasmic photosensitized whole-cell hybrid system, comprising the steps of:

A.选择能够进行细胞周质表达生物酶的细菌细胞接种到对应培养基中,有氧条件下进行活化后,将菌液和培养液(LB/MOPS)按1:100 (v/v)的比例转移至新培养瓶中,待培养基中的细菌浓度(OD600)达到0.4~0.6后,进行厌氧处理使其在细胞周质表达生物酶;A. Select bacterial cells capable of expressing biological enzymes in the periplasm and inoculate them into the corresponding medium. After activation under aerobic conditions, mix the bacterial solution and culture solution (LB/MOPS) at a ratio of 1:100 (v/v) The ratio was transferred to a new culture bottle, and after the bacterial concentration (OD 600 ) in the medium reached 0.4-0.6, anaerobic treatment was performed to express biological enzymes in the periplasm of the cells;

B.待厌氧过程生物酶表达完成之后,在厌氧条件下加入半导体纳米光敏化剂,置于30℃的恒温摇床中进行细胞杂合;B. After the expression of the biological enzyme in the anaerobic process is completed, add a semiconductor nano-photosensitizer under anaerobic conditions, and place it in a constant temperature shaker at 30°C for cell hybridization;

C.杂合完成之后,对溶液进行离心、洗涤,再将细胞周质光敏化的全细胞杂合体系重悬到新的反应缓冲溶液中。C. After the hybridization is completed, the solution is centrifuged and washed, and then the periplasmic photosensitized whole-cell hybrid system is resuspended in a new reaction buffer solution.

本发明较优公开例中,步骤A所述细菌细胞为Shewanella oneidensis,Desulfovibrio gigas, Desulfovibrio vulgaris, Desulfovibrio desulfuricans,Desulfovibrio baculatus In a preferred disclosed example of the present invention, the bacterial cells described in step A are Shewanella oneidensis , Desulfovibrio gigas , Desulfovibrio vulgaris , Desulfovibrio desulfuricans , Desulfovibrio baculatus and the like .

本发明较优公开例中,步骤A所述厌氧处理,其过程为:在超净台中,将菌液转移到500 mL的厌氧瓶中,然后分别加入乳酸、富马酸和半胱氨酸,使其在体系中的浓度分别为20mM、25 mM和10 mM;然后向厌氧瓶中通入氮气30 min,盖上塞子,最外层再用铝盖压实密封,置于30℃摇床,培养20 h。在这个过程中,细菌在厌氧条件下表达出生物酶(氢化酶),通过酶活测定验证酶的活性。当然,针对不同菌种,亦有不同的厌氧处理,需要依据菌种来确定现有技术中的厌氧处理工艺。In the preferred disclosed example of the present invention, the anaerobic treatment described in step A, the process is: in the ultra-clean bench, transfer the bacterial solution to a 500 mL anaerobic bottle, and then add lactic acid, fumaric acid and cysteine respectively acid, so that the concentrations in the system were 20 mM, 25 mM and 10 mM respectively; then nitrogen gas was passed into the anaerobic bottle for 30 min, the stopper was closed, and the outermost layer was compacted and sealed with an aluminum cap, and placed at 30 °C shaker, cultivated for 20 h. In this process, bacteria express biological enzymes (hydrogenases) under anaerobic conditions, and the activity of the enzymes is verified by enzyme activity assays. Of course, there are different anaerobic treatments for different bacterial species, and the anaerobic treatment process in the prior art needs to be determined according to the bacterial species.

本发明较优公开例中,步骤B所述半导体纳米光敏化剂,包括TiO2, NaTaO3,KTaO3, Bi3TaO7, WO3, Bi2O3, BiVO4, CdS纳米粒子, CuIn2S4/ZnS 及 g-C3N4量子点等。可通过X-射线衍射表征所述半导体纳米光敏化剂。粒径过大的纳米粒子会影响细胞的内吞或扩散进入细胞的速率,因此控制纳米粒子的尺寸非常重要。所述半导体纳米光敏化剂颗粒大小以不大于20 nm为宜。In the preferred disclosed example of the present invention, the semiconductor nano-photosensitizer described in step B includes TiO 2 , NaTaO 3 , KTaO 3 , Bi 3 TaO 7 , WO 3 , Bi 2 O 3 , BiVO 4 , CdS nanoparticles, CuIn 2 S 4 /ZnS and gC 3 N 4 quantum dots, etc. The semiconductor nano photosensitizer can be characterized by X-ray diffraction. Nanoparticles that are too large will affect the rate of endocytosis or diffusion into cells, so it is very important to control the size of nanoparticles. The particle size of the semiconductor nano photosensitizer is preferably not greater than 20 nm.

本发明较优公开例中,步骤B中所加入的半导体纳米光敏化剂在杂合体系中的含量为0.25~1.25 mg/mL,保持时间为0.5~2 h。In the preferred disclosed example of the present invention, the content of the semiconductor nano-photosensitizer added in step B in the hybrid system is 0.25-1.25 mg/mL, and the holding time is 0.5-2 h.

其中加入的导体纳米光敏化剂理论含量为1 mg/mL,保持时间为1 h时,细菌内部细胞携带的光敏化剂含量最高,达到28%,光催化产氢效率最好。The theoretical content of the added conductive nano-photosensitizer was 1 mg/mL, and when the holding time was 1 h, the photosensitizer content carried by the cells inside the bacteria was the highest, reaching 28%, and the photocatalytic hydrogen production efficiency was the best.

本发明在步骤A中,以加入甲基紫精和电子供体检测酶活的方法检测氢化酶表达。In step A of the present invention, hydrogenase expression is detected by adding methyl viologen and an electron donor to detect enzyme activity.

本发明的步骤B中,较小的尺寸的纳米粒子或量子点会被细菌细胞逐渐通过内吞作用或扩散作用进入细胞内。含有表面配体的纳米颗粒或量子点被活细胞特异性吸收后,与具有生物识别的分子如肽、抗体、核酸或小分子配体发生化学连接作用。控制半导体纳米光敏化剂的浓度和时间,可以调节进入细胞内的半导体纳米光敏化剂含量的多少。浓度过低时,可扩散或内吞进入细胞的纳米粒子或量子点含量过低,导致纳米粒子或量子点细胞内携带率过低;当纳米粒子或量子点的浓度过高时,纳米粒子或量子点会团聚在一起,也会影响纳米粒子或量子点进入细胞的含量的多少。因此,合理的调控纳米粒子或量子点的浓度和时间,可以使纳米粒子或量子点在细胞中的携带率达到最佳,从而使杂合体系的光催化效率达到最佳。细胞内的光敏化剂的含量通过等离子体电感耦合光谱发生仪(ICP)进行测定。In the step B of the present invention, the smaller-sized nanoparticles or quantum dots will be gradually entered into the cells by the bacterial cells through endocytosis or diffusion. Nanoparticles or quantum dots containing surface ligands are specifically absorbed by living cells, and chemically linked with molecules with biological recognition such as peptides, antibodies, nucleic acids or small molecule ligands. Controlling the concentration and time of the semiconductor nano-photosensitizer can adjust the content of the semiconductor nano-photosensitizer entering the cell. When the concentration is too low, the content of nanoparticles or quantum dots that can diffuse or endocytize into the cell is too low, resulting in a low intracellular carrying rate of nanoparticles or quantum dots; when the concentration of nanoparticles or quantum dots is too high, the nanoparticles or quantum dots Quantum dots will clump together and also affect how much of the nanoparticle or quantum dot gets into the cell. Therefore, rationally adjusting the concentration and time of nanoparticles or quantum dots can optimize the carrying rate of nanoparticles or quantum dots in cells, so that the photocatalytic efficiency of the hybrid system can be optimized. The content of photosensitizer in cells was measured by plasma inductively coupled spectrometer (ICP).

本发明的另外一个目的,在于根据本发明所述方法制得的细胞周质光敏化的全细胞杂合体系,应用于可见光催化制氢。Another object of the present invention is to apply the periplasmic photosensitized whole-cell hybrid system prepared according to the method of the present invention to catalytic hydrogen production with visible light.

CIZS QDs/SW细胞周质光敏化全细胞杂合体系的光催化产氢性能Photocatalytic hydrogen production performance of CIZS QDs/SW periplasmic photosensitized whole-cell hybrid system

使用封闭的气体循环系统测试CIZS QDs/SW细胞周质光敏化全细胞杂合体系的光催化产氢性能。在手套箱中,所制备的杂合体系加入抗坏血酸(100 mM)作为空穴牺牲剂,然后装入反应瓶。采用300W 氙灯的作为光源,紫外光和红外光通过截止滤光片滤掉(420<λ<780 nm)。然后将石英反应器连接到气体循环系统并抽至真空,以确保反应系统处于厌氧状态。使用循环水浴将反应温度控制在37℃。在光照之前,暗反应1小时,以检查设备是否漏气。在室温下进行光催化反应9小时,设定气相色谱自动采样程序,每隔一个小时检测产生的H2的峰面积,并通过气相色谱分析产生H2的含量。The photocatalytic hydrogen production performance of CIZS QDs/SW periplasmic photosensitized whole-cell hybrid system was tested using a closed gas circulation system. In the glove box, the prepared hybrid system was added with ascorbic acid (100 mM) as a cavitation sacrificial agent, and then loaded into a reaction vial. A 300W xenon lamp is used as the light source, and ultraviolet light and infrared light are filtered out by cut-off filters (420<λ<780 nm). The quartz reactor was then connected to a gas circulation system and evacuated to ensure that the reaction system was in an anaerobic state. The reaction temperature was controlled at 37°C using a circulating water bath. React in dark for 1 hour before light to check the device for air leaks. The photocatalytic reaction was carried out at room temperature for 9 hours, the automatic sampling program of gas chromatography was set, the peak area of the generated H2 was detected every hour, and the content of the generated H2 was analyzed by gas chromatography.

为了与单独的光敏化剂的产量进行对比,采用ICP检测了细胞周质光敏化剂全细胞杂合体系中的光敏化剂的浓度,计算出其含量。采用相同的质量的光敏化剂进行实验测定其光催化产氢性能。In order to compare with the output of a single photosensitizer, the concentration of the photosensitizer in the periplasmic photosensitizer whole-cell hybrid system was detected by ICP, and its content was calculated. The photosensitizer with the same quality was used to test its photocatalytic hydrogen production performance.

有益效果Beneficial effect

本发明通过具有广谱吸收范围的半导体纳米粒子与在细胞周质中表达生物酶的细胞来构筑,是一种制备工艺简单,成本低廉,可实现高效太阳能-化学能转化的方法。本发明提出了一种普适性的细胞周质光敏化的全细胞杂合体系的构筑方法,用以实现太阳能-化学能的高效转化,在环境、能源等领域有良好应用前景。The invention is constructed by semiconductor nanoparticles with broad-spectrum absorption range and cells expressing biological enzymes in the periplasm, and is a method with simple preparation process, low cost, and high-efficiency solar-chemical energy conversion. The present invention proposes a method for constructing a universal periplasmic photosensitized whole-cell hybrid system to realize efficient conversion of solar energy to chemical energy, and has good application prospects in the fields of environment and energy.

附图说明Description of drawings

图1. 所制备的CIZS QDs的X-射线衍射图。Figure 1. X-ray diffraction patterns of the as-prepared CIZS QDs.

图2. 所制备的CIZS QDs的透射电镜(a)和高分辨透射图(b)。Figure 2. Transmission electron microscopy (a) and high-resolution transmission image (b) of the as-prepared CIZS QDs.

图3. 所制备的SW的扫描电镜(a)/透射电镜(b)及局部透射电镜图(c)。Figure 3. SEM (a)/TEM (b) and partial TEM image (c) of the prepared SW.

图4. 所构建的CIZS QDs/SW细胞周质光敏化全细胞杂合体系的产氢性能对比图。Figure 4. Comparison of the hydrogen production performance of the constructed CIZS QDs/SW periplasmic photosensitized whole-cell hybrid system.

具体实施方式detailed description

下面结合实施例对本发明进行详细说明,以使本领域技术人员更好地理解本发明,但本发明并不局限于以下实施例。The present invention will be described in detail below in conjunction with the examples, so that those skilled in the art can better understand the present invention, but the present invention is not limited to the following examples.

除非另外限定,这里所使用的术语(包含科技术语)应当解释为具有如本发明所属技术领域的技术人员所共同理解到的相同意义。还将理解到,这里所使用的术语应当解释为具有与它们在本说明书和相关技术的内容中的意义相一致的意义,并且不应当以理想化或过度的形式解释,除非这里特意地如此限定。Unless otherwise defined, terms (including technical and technical terms) used herein should be interpreted as having the same meaning as commonly understood by those skilled in the art to which this invention belongs. It will also be understood that the terms used herein should be interpreted to have a meaning consistent with their meanings in the context of this specification and related art, and should not be interpreted in an idealized or over-the-top form, unless expressly so defined herein .

实施例1Example 1

CIZS QDs/Shewanella oneidensis细胞周质光敏化全细胞杂合体系的构建Construction of CIZS QDs/ Shewanella oneidensis periplasmic photosensitized whole-cell hybrid system

取少量Shewanella oneidensis MR-1(SW)菌种接入到含有含酵母(5 g/L)、胰蛋白胨(10 g/L)和氯化钠(10 g/L)的Luria Bertani(LB)培养基中,置于30°C摇床(180 rpm)有氧条件下过夜培养;然后将100 μL培养液接种到200 mL改良的LB培养基(LB+100 mMMOPS,pH 7.2)中,30°C摇床继续有氧培养3~4 h;通过测量OD600监测细胞生长当细胞浓度(OD600)达到0.4~0.6时,加入20 mM乳酸钠、10 mM半胱氨酸和25 mM富马酸钠,并转移至厌氧血清瓶;用氮气吹洗血清瓶,以除去菌液中的氧气,然后将血清瓶盖上丁基橡胶塞保持密封,置于30°C摇床,厌氧培养20 h。Take a small amount of Shewanella oneidensis MR-1 (SW) and insert it into Luria Bertani (LB) containing yeast (5 g/L), tryptone (10 g/L) and sodium chloride (10 g/L) medium, placed in a 30°C shaker (180 rpm) for overnight culture under aerobic conditions; then inoculated 100 μL of culture solution into 200 mL of modified LB medium (LB+100 mMMOPS, pH 7.2), at 30°C Continue aerobic culture on a shaker for 3-4 h; monitor cell growth by measuring OD 600 . When the cell concentration (OD 600 ) reaches 0.4-0.6, add 20 mM sodium lactate, 10 mM cysteine and 25 mM sodium fumarate, and transferred to an anaerobic serum bottle; the serum bottle was purged with nitrogen to remove the oxygen in the bacterial solution, and then the serum bottle cap was sealed with a butyl rubber stopper, and placed on a shaker at 30°C for anaerobic incubation for 20 h.

待上述在厌氧培养中完成后,将100 mg CIZS QDs加入(厌氧条件)到SW细胞菌液培养基中,额外厌氧培养1小时,以确保CIZS QD被SW携带进入细胞内部。最后将细胞菌液培养基离心5分钟,转速5000 rpm,洗涤,收集细胞沉淀并重悬于Tris缓冲液中,从而得到CIZSQDs/SW细胞周质光敏化全细胞杂合体系。After the above-mentioned anaerobic culture was completed, 100 mg CIZS QDs were added (anaerobic conditions) to the SW cell culture medium, and an additional anaerobic culture was performed for 1 hour to ensure that the CIZS QDs were carried by the SW into the cell interior. Finally, the cell culture medium was centrifuged at 5000 rpm for 5 minutes, washed, and the cell pellet was collected and resuspended in Tris buffer to obtain the CIZSQDs/SW periplasmic photosensitized whole-cell hybrid system.

所制得CIZS QDs/SW细胞周质光敏化全细胞杂合体系内部细胞携带的光敏化剂含量28%,可见光下反应9 h产氢效率为490μmol。The prepared CIZS QDs/SW periplasmic photosensitized whole-cell hybrid system contained 28% of the photosensitizer carried by the internal cells, and the hydrogen production efficiency was 490 μmol after 9 hours of reaction under visible light.

实施例2Example 2

CIZS QDs/Desulfovibrio vulgaris细胞周质光敏化全细胞杂合体系的构建Construction of CIZS QDs/ Desulfovibrio vulgaris periplasmic photosensitized whole-cell hybrid system

取少量Desulfovibrio vulgaris菌种接入到碳酸氢盐缓冲培养基,此培养基中包含酵母粉、蛋白胨、微量矿物质、维生素、NaH2CO3、 NH4Cl、NaH2PO4、KCl、60% 乳酸糖浆、MgSO4、Na2SO4,加入乳酸和和柠檬酸铁(III)分别作为电子供体和电子受体,置于35°C摇床(180 rpm)有氧条件下过夜培养;随后将100 mg CIZS QDs加入到Desulfovibrio vulgaris,额外厌氧培养1小时,以确保CIZS QD被Desulfovibrio vulgaris携带进入细胞内部;最后将细胞菌液培养基离心5分钟,转速5000 rpm,洗涤,收集细胞沉淀并重悬于碳酸氢盐缓冲液中,从而得到CIZS QDs/Desulfovibrio vulgaris细胞周质光敏化全细胞杂合体系。Take a small amount of Desulfovibrio vulgaris strain and insert it into bicarbonate buffer medium, which contains yeast powder, peptone, trace minerals, vitamins, NaH 2 CO 3 , NH 4 Cl, NaH 2 PO 4 , KCl, 60% Add lactic acid syrup, MgSO 4 , Na 2 SO 4 , add lactic acid and iron (III) citrate as electron donor and electron acceptor respectively, and culture overnight under aerobic conditions at 35°C on a shaker (180 rpm); then Add 100 mg CIZS QDs to Desulfovibrio vulgaris and incubate anaerobically for an additional 1 hour to ensure that CIZS QDs are carried by Desulfovibrio vulgaris into the cell; finally, centrifuge the cell culture medium at 5000 rpm for 5 minutes, wash, collect the cell pellet and re- Suspended in bicarbonate buffer to obtain CIZS QDs/ Desulfovibrio vulgaris periplasmic photosensitized whole-cell hybrid system.

所制得CIZS QDs/Desulfovibrio vulgaris细胞周质光敏化全细胞杂合体系内部细胞携带的光敏化剂含量23%,可见光下反应9 h产氢效率为426μmol。The prepared CIZS QDs/ Desulfovibrio vulgaris periplasmic photosensitized whole-cell hybrid system contained 23% of the photosensitizer carried by the internal cells, and the hydrogen production efficiency was 426 μmol after 9 hours of reaction under visible light.

实施例3Example 3

CdS/Desulfovibrio gigas细胞周质光敏化全细胞杂合体系的构建Construction of CdS/ Desulfovibrio gigas periplasmic photosensitized whole-cell hybrid system

取少量Desulfovibrio gigas菌种接入到含有乳酸和硫酸盐作为碳和能源的培养基中,置于35℃摇床(180 rpm)有氧条件下过夜培养;测量OD600监测细胞生长,待细胞达到指数生长后期,将100 mg CdS加入(厌氧条件)到Desulfovibrio gigas细胞菌液培养基中,额外厌氧培养1小时,以确保CdS被Desulfovibrio gigas携带进入细胞内部;最后将细胞菌液培养基离心5分钟,转速5000 rpm,洗涤,收集细胞沉淀并重悬于MOPS缓冲液中,从而得到CdS/Desulfovibrio gigas细胞周质光敏化全细胞杂合体系。Take a small amount of Desulfovibrio gigas strains and insert them into the medium containing lactic acid and sulfate as carbon and energy sources, and place them on a shaker (180 rpm) at 35°C for overnight culture under aerobic conditions; measure OD 600 to monitor cell growth, and wait until the cells reach In the late stage of exponential growth, add 100 mg CdS (anaerobic conditions) to the Desulfovibrio gigas cell culture medium and incubate anaerobically for an additional 1 hour to ensure that CdS is carried by Desulfovibrio gigas into the cell interior; finally, the cell culture medium is centrifuged Wash at 5000 rpm for 5 minutes, collect the cell pellet and resuspend in MOPS buffer to obtain a CdS/ Desulfovibrio gigas periplasmic photosensitized whole-cell hybrid system.

所制得CdS/Desulfovibrio gigas细胞周质光敏化全细胞杂合体系内部细胞携带的光敏化剂含量18%,可见光下反应9 h产氢效率为386μmol。The prepared CdS/ Desulfovibrio gigas periplasmic photosensitized whole-cell hybrid system contained 18% of the photosensitizer carried by the internal cells, and the hydrogen production efficiency was 386 μmol after 9 hours of reaction under visible light.

以上所述仅为本发明的实施例,并非因此限制本发明的专利范围,凡是利用本发明说明书所作的等效结构或等效流程变换,或直接或间接运用在其他相关的技术领域,均同理包括在本发明的专利保护范围内。The above is only an embodiment of the present invention, and does not limit the patent scope of the present invention. Any equivalent structure or equivalent process transformation made by the description of the present invention, or directly or indirectly used in other related technical fields, shall be the same as The theory is included in the patent protection scope of the present invention.

Claims (5)

1. A method for constructing a periplasmic photosensitized whole-cell hybrid system, comprising the steps of:
A. selecting Shewanella oneidensis MR-1 capable of expressing biological enzyme in periplasm of cells, inoculating into corresponding culture medium, activating under aerobic condition, inoculating the culture solution into improved LB culture medium until the bacterial concentration OD in the culture medium 600 After reaching 0.4-0.6, anaerobic treatment is carried out to enable the bacteria to express biological enzyme in the periplasm of the cells;
B. after the biological enzyme expression in the anaerobic process is finished, adding a semiconductor nano photosensitizer CuInS under the anaerobic condition 2 ZnS, placing in a constant temperature shaking table at 30 ℃ for cell hybridization;
C. after the hybridization is finished, centrifuging and washing the solution, and then re-suspending the whole-cell hybridization system with the photosensitization of the periplasm into a new reaction buffer solution;
the anaerobic treatment of the step A comprises the following steps: transferring the bacterial liquid into a 500mL anaerobic bottle in a super clean bench, and then respectively adding lactic acid, fumaric acid and cysteine to make the concentrations of the lactic acid, the fumaric acid and the cysteine in a system respectively 20mM, 25mM and 10mM; then introducing nitrogen into the anaerobic bottle for 30min, covering a plug, compacting and sealing the outermost layer by using an aluminum cover, placing the anaerobic bottle in a shaking table at 30 ℃, and culturing for 20h.
2. The method of constructing a periplasmic photosensitized whole cell hybrid system according to claim 1, wherein: and B, the particle size of the semiconductor nano photosensitizer is not more than 20nm.
3. The method of constructing a periplasmic photosensitized whole cell hybrid system according to claim 1, wherein: the content of the semiconductor nano photosensitizer added in the step B in the hybrid system is 0.25-1.25 mg/mL, and the retention time is 0.5-2 h.
4. A whole cell hybrid system with photosensitization of periplasm of cells constructed according to the method of any one of claims 1 to 3.
5. Use of a periplasmic photosensitized whole cell hybrid system according to claim 4, wherein: the catalyst is applied to visible light catalysis hydrogen production.
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