Chromatofocusing of peptides and proteins using linear pH gradients formed on strong ion‐exchange adsorbents

Kang, Xuezhen; Frey, Douglas D.

doi:10.1002/bit.20122

Cited by 27 publications

(14 citation statements)

References 24 publications

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“…Due to technically limited resolution of the pH-gradient [28], a wide peak base was observed. Kang and Frey [37] compared different column packing of strong and weak ion-exchange adsorbents for chromatofocusing with regard to the linearity of the pH-gradient and resolution. It was reported that strong ion-exchange adsorbents could achieve the same or even slightly better resolutions.…”

Section: Discussionmentioning

confidence: 99%

Reducing sample complexity of polyclonal human autoantibodies by chromatofocusing

Hagemann

Faude

Rabenstein

et al. 2010

Journal of Chromatography B

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Section: Discussionmentioning

confidence: 99%

Reducing sample complexity of polyclonal human autoantibodies by chromatofocusing

Hagemann

Faude

Rabenstein

et al. 2010

Journal of Chromatography B

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“…alternatively, the ProteomeLab PF2D platform (Beckman Coulter, USA) used for the quantitative comparisons and separation/fractionation of various biological and clinical samples, works in full automation combining chromatofocusing separation and hydrophobic fractionation 47 . During the first-dimension chromatofocusing of PF2D, proteins are first separated by their pI and then separated proteins with a pH gradient are collected using a fraction collector 48,49 . Subsequently, in the second dimension, the collected fractions from the first dimension are separated using reversed phase chromatography which works on the basis of hydrophobicity 49 .…”

Section: Automated Proteomic Analysis Using Proteomelab Pf2d Platformmentioning

confidence: 99%

Toxicoproteomic approaches for analysis of microbial community inhabiting Asian dust particles

Sekhon

Ahn

Min

et al. 2015

Mol. Cell. Toxicol.

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in this review, we provide an overview of the bio-analytical approaches for proteomic analysis of asian dust storms. asian dust has been known to travel with high-speed eastward winds and affects air quality over Japan and even the western coast of the U.S. during severe occurrences. Several reports have shown that asian dust particles have a negative effect on a wide range of industries and human health activities. Here we give a short overview of asian dust feature and its proteomic analysis approaches including 2-De PaGe, metaproteomic analysis of large environmental samples, and automatic techniques for dust microbial analysis. Following this, we discuss the detection system of asian dust particles that can be integrated with biosensor platform.

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“…Se utilizó el sistema de rotofor (Biorad, Richmond, Estados Unidos) para separar las proteínas por punto isoeléctrico (42). La fracción correspondiente a las proteínas asociadas con membrana se preparó así: 2,5 ml de muestra, 1 ml de anfolitos con rango de pH de 3 a 10, 3 ml de glicerol estéril y 11,5 ml de agua miliq estéril.…”

Section: Separación De Proteínas Por Punto Isoeléctricounclassified

Producción y purificación de la proteína core del virus de la hepatitis C en el sistema de expresión del baculovirus para ensayos biológicos.

Rubio¹,

Cómbita²,

Ortiz-Reyes³

et al. 2005

biomedica

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Introducción. La infección por el virus de la hepatitis C (VHC) se caracteriza por la alta frecuencia de infección persistente. La capacidad del VHC para inducir alteraciones en la función de las células del sistema inmune, específicamente en las células dendríticas, parece ser una de las estrategias virales implicada en el establecimiento de la infección persistente. Esta estrategia parece estar mediada en gran parte por una de las proteínas estructurales codificada por el genoma del VHC, la proteína Core, unidad estructural de la cápside viral. Objetivo. Una de las limitantes para la evaluación de las propiedades de Core es la obtención y la purificación de la proteína nativa (191 aa). El objetivo de este estudio fue la producción y la purificación de la proteína Core completa en un sistema eucariote para evaluar las propiedades de la proteína en cultivos de células dendríticas humanas. Resultados. En este estudio se logró la producción de la proteína Core completa en el sistema de expresión de baculovirus y su purificación por la técnica de separación por punto isoeléctrico y electroelución. La pureza de la proteína obtenida se confirmó por Western blot y tinción con plata. Estos análisis mostraron dos bandas únicas correspondientes a las isoformas p23 y p21 de la proteína Core, previamente descritas en la literatura. Conclusiones. La proteína obtenida posee varias de las condiciones de la proteína Core nativa, como peso molecular, isoformas y localización subcelular. Los procedimientos descritos en este artículo son aplicables a proteínas asociadas a membranas producidas en sistemas de expresión eucarióticos. Palabras clave: virus de la hepatitis C, proteína Core, Baculovirus, sistema de expresión, isoelectroenfoque, purificación.Hepatitis C virus core protein production and purification in a baculovirus expression system for biological assays Background. The hepatitis C virus (HCV) commonly causes persistent infection. One of the viral mechanisms in preventing viral clearance is the ability of HCV to induce functional alterations of the immune system cells, specifically of dendritic cells. Viral proteins producing the dendritic cell functional alterations have been identified as the HCV core protein, which makes up the capsid structural unit. Objective. One of the limitations to evaluate core protein properties is the difficulty in obtaining and purifying the complete protein -consisting of 191 amino acids. The aim of the current study was to produce and purify the recombinant core protein in a eukaryotic system, and to evaluate its effect in human dendritic cell cultures. Results. The core protein p23 isoform was expressed in a baculovirus system and purified using isoelectric point separation and electroelution. The purity of the core protein was confirmed by silver stain and Western blot. These analyses showed the presence of two bands that correspond to p23 and p21 isoforms of core protein as previously reported. Conclusion. The expressed protein differed from naive core protein is terms of molecular we...

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Chromatofocusing of peptides and proteins using linear pH gradients formed on strong ion‐exchange adsorbents

Cited by 27 publications

References 24 publications

Reducing sample complexity of polyclonal human autoantibodies by chromatofocusing

Reducing sample complexity of polyclonal human autoantibodies by chromatofocusing

Toxicoproteomic approaches for analysis of microbial community inhabiting Asian dust particles

Producción y purificación de la proteína core del virus de la hepatitis C en el sistema de expresión del baculovirus para ensayos biológicos.

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