| Expression and Purification of Arabidopsis Transmembrane Protein BCM1 in Saccharomyces cerevisiae
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Author:
Date:
2020-09-20
[Abstract] Heterologous expression and purification of transmembrane proteins have remained a challenge for decades hampering detailed biochemical and structural characterization of key enzymes and their interacting regulators in multiple metabolic pathways. An in-depth study on the newly identified Arabidopsis thaliana integral membrane protein BALANCE OF CHLOROPHYLL METABOLISM 1 (BCM1) showed a stimulatory effect of the BCM1 on magnesium chelatase, the first enzyme of chlorophyll biosynthesis, through interaction with the GENOMES UNCOUPLED 4 (Wang et al., 2020). Here, we report a detailed and optimized method for heterologous expression and purification of His-tagged BCM1 in Saccharomyces cerevisiae. Following this method, we obtained native BCM1 used for in vitro ...
[摘要] [摘要 ] 异源表达和公顷跨膜蛋白的纯化VE 仍然几十年来阻碍了关键酶详述生物化学和结构表征一个挑战小号和它们的相互作用调节在多个代谢途径。上新鉴定进行了深入的研究拟南芥拟南芥叶绿素代谢1(BCM1)的整合膜蛋白BALANCE显示一个通过与相互作用对镁螯合,叶绿素生物合成的第一个酶,所述BCM1的刺激效应基因组中脱开4 (王等等人,2020)。这里 ,我们报告了酿酒酵母中His-tagged BCM1异源表达和纯化的详细和优化方法。˚F ollowing这种方法,我们获得用于本机BCM1 体外酶测定的镁螯合(王等人,2020) 。目前,BCM1的结晶研究正在进行中。这个协议可以适于纯化BCM 1一样从用于酶和结构研究真核生物的跨膜蛋白。
[背景 ] 鉴定翻译后单组的lators其指导LY 调制enzym 一个叶绿素合成的酶的抽动活动可以大大提高我们理解的分子机制,通过该植物保持高效叶绿素叶期间LL合成绿化(Brzezowski 等人,2015年)。然而,叶绿素合成酶及其相互作用蛋白的详细生化分析受到体外重组蛋白可用性的限制。我们最近发现一个叶绿素代谢1(BCM1)的翻译后调节平衡,同时刺激小号叶绿素合成和延迟叶绿素分解,日ERE 被授予叶发育过程中的叶绿素稳态(王等人,2020年)。为了检查BCM1对镁螯合酶(MgCh ...
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| Assessing in vitro and in vivo Trogocytosis By Murine CD4+ T cells
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Author:
Date:
2020-05-05
[Abstract] Recognition of antigens by lymphocytes (B, T, and NK) on the surface of an antigen-presenting cell (APC) leads to lymphocyte activation and the formation of an immunological synapse between the lymphocyte and the APC. At the immunological synapse APC membrane and associated membrane proteins can be transferred to the lymphocyte in a process called trogocytosis. The detection of trogocytosed molecules provides insights to the activation state, antigen specificity, and effector functions and differentiation of the lymphocytes. Here we outline our protocol for identifying trogocytosis-positive CD4+ T cells in vitro and in vivo. In vitro, antigen presenting cells are surface biotinylated and pre-loaded with magnetic polystyrene beads before incubating for ...
[摘要] [摘要 ] 抗原呈递细胞(APC)表面的淋巴细胞(B,T和NK)识别抗原会导致淋巴细胞活化并在淋巴细胞和APC之间形成免疫突触。在免疫突触处APC膜和相关的膜蛋白可以转移调用Trogocytosis到淋巴细胞的过程。检测Trogocytosed分子提供见解的激活状态,抗原特异性和效应器功能和差异的淋巴细胞。这里我们列出了我们的协议,用于识别Trogocytosis CD4阳性Tasu 性T细胞在体外和体内。体外,抗原呈递细胞是表面 生物素化并预装磁性聚苯乙烯珠,然后与体外活化的CD4 + T细胞胚细胞(90分钟)或幼稚T细胞(3-24小时)短时间孵育。阳性(trog + )细胞可通过链霉亲和素染色来筛选经生物素化的经转钙蛋白的APC膜蛋白,然后立即或在随后的孵育后通过流式细胞仪分析其激活表型,效应子功能和效应子的分化,例如,可以鉴定出嗜光细胞的阳性细胞。以前的研究已经描述了分析T细胞嗜光性的方法,以鉴定抗原特异性细胞或被细胞识别的抗原表位。使用当前方案,嗜光性对单个T细胞的影响或能力trog + T细胞调节其他免疫细胞的激活和功能的能力可在一个扩展范围内进行评估 ed时间段。
[背景 ] Trogocytosis是质膜和膜相关分子的细胞间转移。这种现象已在免疫细胞相互作用的分析中得到了广泛研究,并已观察到包括向CD4 +的转移(Wetzel 等,2005; ...
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