4.7 Article

Capillary Sodium Dodecyl Sulfate Agarose Gel Electrophoresis of Proteins

期刊

GELS
卷 8, 期 2, 页码 -

出版社

MDPI
DOI: 10.3390/gels8020067

关键词

capillary electrophoresis; agarose; SDS-protein complexes; therapeutic antibody

资金

  1. National Research, Development and Innovation Office [2018-2.1.17-TET-KR-2018-00010]
  2. New National Excellence Program of the Ministry for Innovation and Technology of Hungary [UNKP-21-3-II-DE-276]

向作者/读者索取更多资源

This paper introduces a new capillary agarose gel electrophoresis method for the separation of low molecular weight immunoglobulin subunits. Through adjusting the concentration of agarose and boric acid, the sieving performance of the gel was optimized, achieving good resolution and separation power. Additionally, this method does not require capillary regeneration steps, saving analysis time.
Capillary sodium dodecyl sulfate gel electrophoresis has long been used for the analysis of proteins, mostly either with entangled polymer networks or translationally cross-linked gels. In this paper capillary agarose gel electrophoresis is introduced for the separation of low molecular weight immunoglobulin subunits. The light (LC similar to 24 kDa) and heavy (HC similar to 50 kDa) chain fragments of a monoclonal antibody therapeutic drug were used to optimize the sieving matrix composition of the agarose/Tris-borate-EDTA (TBE) systems. The agarose and boric acid contents were systematically varied between 0.2-1.0% and 320-640 mM, respectively. The influence of several physical parameters such as viscosity and electroosmotic flow were also investigated, the latter to shed light on its effect on the electrokinetic injection bias. Three dimensional Ferguson plots were utilized to better understand the sieving performance of the various agarose/TBE ratio gels, especially relying on their slope (retardation coefficient, K-R) value differences. The best resolution between the LC and non-glycosylated HC IgG subunits was obtained by utilizing the molecular sieving effect of the 1% agarose/320 mM boric acid composition (Delta K-R = 0.035). On the other hand, the 0.8% agarose/640 mM boric acid gel showed the highest separation power between the similar molecular weight, but different surface charge density non-glycosylated HC and HC fragments (Delta K-R = 0.005). It is important to note that the agarose-based gel-buffer systems did not require any capillary regeneration steps between runs other than simple replenishment of the sieving matrix, significantly speeding up analysis cycle time.

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