Literature DB >> 15692460

Specific interaction between lens MIP/Aquaporin-0 and two members of the gamma-crystallin family.

Jianguo Fan1, Robert N Fariss, Andrew G Purkiss, Christine Slingsby, Aileen Sandilands, Roy Quinlan, Graeme Wistow, Ana B Chepelinsky.   

Abstract

PURPOSE: Major Intrinsic Protein (MIP)/Aquaporin 0 is required for lens transparency and is specifically expressed in lens fiber cell membranes. We have demonstrated previously that in the rat lens MIP interacts specifically with gammaE-crystallin, resulting in its recruitment to the plasma membrane. Our goal was to examine the interaction or lack of interaction between MIP and all members of the gamma-crystallin family and to provide evidence for a physiological role these interactions may play in gamma-crystallin or MIP function.
METHODS: Full length MIP was expressed as untagged, enhanced green fluorescent protein (EGFP) tagged, or myc tagged proteins. Members of the gamma-crystallin family were expressed as red fluorescent protein (HcRed) tagged proteins in the rabbit kidney epithelial cell line RK13. Co-localization of tagged proteins was analyzed by confocal fluorescence microscopy.
RESULTS: Confocal fluorescence microscopy demonstrated that gammaE- and gammaF-crystallin co-localize specifically with full length MIP in mammalian cells while other gamma-crystallins, including gammaA-, gammaB-, gammaC-, gammaD-, and gammaS-crystallin do not. As a result of this interaction, either gammaE- or gammaF-crystallin was recruited to the plasma membrane from the cytoplasm. MIP does not interact with the Elo mutant of gammaE-crystallin, which has been linked to a dominant cataract phenotype in mice.
CONCLUSIONS: These experiments demonstrate that MIP interacts selectively with gammaE- and gammaF-crystallin, and not with other gamma-crystallins. This raises the possibility of MIP playing a structural role in the organization of gamma-crystallins in rodent lens fibers and/or that gammaE- and gammaF-crystallin may have a specific role in MIP function in the rodent lens.

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Year:  2005        PMID: 15692460

Source DB:  PubMed          Journal:  Mol Vis        ISSN: 1090-0535            Impact factor:   2.367


  15 in total

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2.  Endogenous retroviral insertion in Cryge in the mouse No3 cataract mutant.

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Authors:  Shuhua Song; Andrew Landsbury; Ralf Dahm; Yizhi Liu; Qingjiong Zhang; Roy A Quinlan
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4.  Two distinct aquaporin 0s required for development and transparency of the zebrafish lens.

Authors:  Alexandrine Froger; Daniel Clemens; Katalin Kalman; Karin L Németh-Cahalan; Thomas F Schilling; James E Hall
Journal:  Invest Ophthalmol Vis Sci       Date:  2010-07-29       Impact factor: 4.799

5.  Functional expression of aquaporins in embryonic, postnatal, and adult mouse lenses.

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6.  Aquaporin 0 enhances gap junction coupling via its cell adhesion function and interaction with connexin 50.

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7.  A novel mutation in the major intrinsic protein (MIP) associated with autosomal dominant congenital cataracts in a Chinese family.

Authors:  Wei Wang; Jin Jiang; Yanan Zhu; Jinyu Li; Chongfei Jin; Xingchao Shentu; Ke Yao
Journal:  Mol Vis       Date:  2010-03-25       Impact factor: 2.367

8.  Expression profiling after retinal detachment and reattachment: a possible role for aquaporin-0.

Authors:  Rafal Farjo; Ward M Peterson; Muna I Naash
Journal:  Invest Ophthalmol Vis Sci       Date:  2008-02       Impact factor: 4.799

9.  Lengsin expression and function during zebrafish lens formation.

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Journal:  Exp Eye Res       Date:  2008-03-02       Impact factor: 3.467

10.  Major intrinsic protein (MIP) polymorphism is associated with age-related cataract in Chinese.

Authors:  Zhou Zhou; Binbin Wang; Yongfeng Luo; Guangkai Zhou; Shanshan Hu; Han Zhang; Xu Ma; Yanhua Qi
Journal:  Mol Vis       Date:  2011-08-25       Impact factor: 2.367

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