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Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection.

Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Research Abstract Details 

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  • Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Abstract Text:

    sung ho parkSung Ho Park,cheolho cheongCheolho Cheong,juliana idoyagaJuliana Idoyaga,jae y kimJae Y Kim,jae-hoon choiJae-Hoon Choi,yoonkyung doYoonkyung Do,haekyung leeHaekyung Lee,jung heon joJung Heon Jo,yong-seok ohYong-Seok Oh,wonpil imWonpil Im,ralph m steinmanRalph M Steinman,chae gyu parkChae Gyu Park,

    Previously, we prepared monoclonal antibodies (mAbs) by immunizing rats with the recombinant fusion proteins of mouse Langerin/CD207, which contained a flexible linker sequence from E. coli OmpF and a FLAG epitope. We found many of new rat mAbs were not reactive to mouse Langerin, and here we identify the epitopes of two of these IgG mAbs, L2 and L5, and assess their efficacy in various immunodetection methods. MAb L5 is a rat IgG mAb against the FLAG epitope, which detected both N-terminal and C-terminal FLAG tagged protein 2 to 8 times better than the conventional anti-FLAG mAb M2 by Western blot. For mAb L2, we found its epitope to be a 14 amino acid sequence SGFANELGPRLMGK which consisted of both sequences from the OmpF derived linker and mouse Langerin. This epitope sequence was named OLLAS (E. coliOmpF Linker and mouse Langerin fusion Sequence), and mAb L2 as mAb OLLA-2. When the OLLAS sequence was inserted into recombinant proteins at N-terminal, C-terminal, or internal sites, the OLLAS tag was detected by mAb OLLA-2 with very high sensitivity compared to other conventional epitope tags and anti-tag mAbs. MAb OLLA-2 recognized OLLAS tagged proteins with at least 100-fold more sensitivity than anti-FLAG M2 and anti-V5 mAbs in Western blot analyses. We also find the OLLAS epitope to be superior in immunoprecipitation and other immunodetection methods, such as fluorescent immunohistochemistry and flow cytometry. In the process, we successfully utilized the OLLAS epitope sequence as an internal linker for fusion between the engineered mAb and the antigen, and thus achieved improved immunodetection.

    Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Publishing Authors By Initials

    sh parkSH Park,c cheongC Cheong,j idoyagaJ Idoyaga,jy kimJY Kim,jh choiJH Choi,y doY Do,h leeH Lee,jh joJH Jo,ys ohYS Oh,w imW Im,rm steinmanRM Steinman,cg parkCG Park,

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    Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Journal Published:

    PUBLICATION TYPE: Journal Article

    Journal: Journal of immunological methods

    VOLUME: 331

    Page Numbers: 27-38

    Journal Abbreviation: J. Immunol. Methods

    ISSN: 0022-1759

    DAY: 26

    MONTH: 11

    YEAR: 2007

    Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Information

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    LANGUAGE: eng

    NlmUniqueID: 1305440

    Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection. Keywords Mesh Terms:

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    Grant and Affiliation Information for Generation and application of new rat monoclonal antibodies against synthetic FLAG and OLLAS tags for improved immunodetection.

    AFFILIATION: Laboratory of Cellular Physiology and Immunology and Chris Browne Center for Immunology and Immune Diseases, The Rockefeller University, 1230 York Avenue, New York, New York 10065, USA.

    Country: Netherlands

    Netherlands Research PublicationNetherlands Research Publication

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    MEDLINETA: J Immunol Methods

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