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首页> 美国卫生研究院文献>Technology in Cancer Research Treatment >Sensitive Detection of Immunoglobulin G Stability Using in Real-Time Isothermal Differential Scanning Fluorimetry: Determinants of Protein Stability for Antibody-Based Therapeutics
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Sensitive Detection of Immunoglobulin G Stability Using in Real-Time Isothermal Differential Scanning Fluorimetry: Determinants of Protein Stability for Antibody-Based Therapeutics

机译:实时等温差示扫描荧光法灵敏检测免疫球蛋白G稳定性:基于抗体的治疗药物的蛋白质稳定性的决定因素

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Protein instability is a major obstacle in the production and delivery of monoclonal antibody–based therapies for cancer. This study presents real-time isothermal differential scanning fluorimetry as an emerging method to evaluate the stability of human immunoglobulin G protein with high sensitivity. The stability of polyclonal human immunoglobulin G against urea-induced denaturation was assessed following: (1) oxidation by the free-radical generator 2,2-Azobis[2-amidinopropane]dihydrochloride and (2) in selected storage buffers. Significant differences in immunoglobulin G stability were detected by real-time isothermal differential scanning fluorimetry when the immunoglobulin G was stored in 1,4-Piperazinediethanesulfonic acid buffer compared to phosphate-buffered saline, with half-maximal rate of denaturation occurring at a higher urea concentration in 1,4-Piperazinediethanesulfonic acid than phosphate-buffered saline (K nd;PIPES = 3.56 ± 0.09 M, K nd;PBS = 2.94 ± 0.08 M; P < .01), but differential scanning fluorimetry did not detect differences in unfolding temperature (T m;PIPES = 70.5 ± 0.3°C, T m;PBS = 69.7 ± 0.2°C). The effects of 2,2-Azobis[2-amidinopropane]dihydrochloride-induced oxidation on immunoglobulin G stability were analyzed by real-time isothermal differential scanning fluorimetry; the oxidized protein showed greater sensitivity to urea (K nd;CNTRL = 3.96 ± 0.19 M, K nd;AAPH = 3.49 ± 0.07 M; P < .05). Similarly, differential scanning fluorimetry indicated greater thermal sensitivity of oxidized immunoglobulin G (T m;CNTRL = 70.5 ± 0.3°C, T m;AAPH = 62.9 ± 0.1°C; P < .001). However, a third method for assessing protein stability, pulse proteolysis, proved to be substantially less sensitive and did not detect significant effects of 2,2-Azobis[2-amidinopropane]dihydrochloride on the half-maximal concentration of urea needed to denature immunoglobulin G (C m;CNTRL= 6.8 ± 0.1 M; C m;AAPH = 6.4 ± 0.7 M). Overall these results demonstrate the merit of using real-time isothermal differential scanning fluorimetry as a rapid and sensitive technique for the evaluation of protein stability in solution using a quantitative real-time thermocycler.
机译:蛋白质不稳定性是基于单克隆抗体的癌症疗法的生产和交付的主要障碍。这项研究提出了实时等温差示扫描荧光法作为一种新兴的方法来评估人类免疫球蛋白G蛋白具有高灵敏度的稳定性。评估多克隆人免疫球蛋白G对尿素诱导的变性的稳定性:(1)由自由基生成剂2,2-偶氮双[2-ami基丙烷]二盐酸盐氧化,以及(2)在选定的存储缓​​冲液中氧化。当将免疫球蛋白G储存在1,4-哌嗪二乙烷磺酸缓冲液中(与磷酸盐缓冲液相比)时,通过实时等温差示扫描荧光法检测到了免疫球蛋白G稳定性的显着差异,在较高的尿素浓度下变性的最大速率发生了一半1,4-哌嗪二乙烷磺酸中的盐含量高于磷酸盐缓冲液(K nd; PIPES = 3.56±0.09 M,K nd; PBS = 2.94±0.08 M; P <.01),但差示扫描荧光法未检测到展开温度的差异(T m; PIPES = 70.5±0.3℃,T m; PBS = 69.7±0.2℃)。实时等温差示扫描荧光法分析了2,2-偶氮双[2-ami基丙烷]二盐酸盐诱导的氧化对免疫球蛋白G稳定性的影响。氧化蛋白对尿素的敏感性更高(K nd; CNTRL = 3.96±0.19 M,K nd; AAPH = 3.49±0.07 M; P <.05)。类似地,差示扫描荧光法表明氧化的免疫球蛋白G具有更高的热敏性(T m; CNTRL = 70.5±0.3°C,T m; AAPH = 62.9±0.1°C; P <.001)。但是,第三种评估蛋白质稳定性的方法,即脉冲蛋白水解,被证明实质上不那么敏感,并且没有检测到2,2-偶氮二[2-ami基丙烷]二盐酸盐对使免疫球蛋白G变性所需的尿素半数最大浓度的显着影响。 (C m; CNTRL = 6.8±0.1M; C m; AAPH = 6.4±0.7M)。总体而言,这些结果证明了使用实时等温差示扫描荧光法作为一种快速,灵敏的技术,可以使用定量实时热循环仪评估溶液中蛋白质的稳定性。

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