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Literature DB >> 2472401

Conformational change of rabbit aminopeptidase N into enterocyte plasma membrane domains analyzed by flow cytometry fluorescence energy transfer.

J P Gorvel¹, Z Mishal, F Liegey, A Rigal, S Maroux.

Abstract

Membrane vesicle preparations are very appropriate material for studying the topology of glycoproteins integrated into specialized plasma membrane domains of polarized cells. Here we show that the flow cytometric measurement of fluorescence energy transfer used previously to study the relationship between surface components of isolated cells can be applied to membrane vesicles. The fluorescein and rhodamine derivatives of a monoclonal antibody (4H7.1) that recognized one common epitope of the rabbit and pig aminopeptidase N were used for probing the oligomerization and conformational states of the enzyme integrated into the brush border and basolateral membrane vesicles prepared from rabbit and pig enterocytes. The high fluorescent energy transfer observed in the case of pig enzyme integrated into both types of vesicles and in the case of the rabbit enzyme integrated into basolateral membrane vesicles agreed very well with the existence of a dimeric organization, which was directly demonstrated by cross-linking experiments. Although with the latter technique we observed that the rabbit aminopeptidase was also dimerized in the brush border membrane, no energy transfer was detected with the corresponding vesicles. This indicates that the relative positions of two associated monomers differ depending on whether the rabbit aminopeptidase is transiently integrated into the basolateral membrane or permanently integrated into the brush border membrane. Cross-linking of aminopeptidases solubilized by detergent and of their ectodomains liberated by trypsin showed that only interactions between anchor domains maintained the dimeric structure of rabbit enzyme whereas interactions between ectodomains also exist in the pig enzyme. This might explain why the noticeable change in the organization of the two ectodomains observed in the case of rabbit aminopeptidase N does not occur in the case of pig enzyme.

Entities: Chemical Gene Species

Mesh：

Substances：

Year: 1989 PMID： 2472401 PMCID： PMC2115577 DOI： 10.1083/jcb.108.6.2193

Source DB: PubMed Journal: J Cell Biol ISSN： 0021-9525 Impact factor: 10.539

42 in total

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Review 4. Mutations that influence the secretory path in animal cells.

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5. Identification of glycoproteins bearing human blood group A determinants in rabbit enterocyte plasma membranes.

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Conformational change of rabbit aminopeptidase N into enterocyte plasma membrane domains analyzed by flow cytometry fluorescence energy transfer.

1. Proximity of lectin receptors on the cell surface measured by fluorescence energy transfer in a flow system.

Review 2. The class II molecules of the human and murine major histocompatibility complex.

Review 3. Fluorescence polarization assay by flow cytometry.

Review 4. Mutations that influence the secretory path in animal cells.

5. Identification of glycoproteins bearing human blood group A determinants in rabbit enterocyte plasma membranes.

6. Biosynthesis of the IgA antibody receptor: a model for the transepithelial sorting of a membrane glycoprotein.

7. Flow cytometric measurement of fluorescence resonance energy transfer on cell surfaces. Quantitative evaluation of the transfer efficiency on a cell-by-cell basis.

8. Molecular identification of receptors for vasoactive intestinal peptide in rat intestinal epithelium by covalent cross-linking. Evidence for two classes of binding sites with different structural and functional properties.

9. Dual parameter, quantitative cytofluorometric analysis of endogenous H-2Kk and foreign HLA class I molecules expressed at the surface of murine transformed L cells.

10. Distribution and mobility of murine histocompatibility H-2Kk antigen in the cytoplasmic membrane.

1. Structure and activity of CPNGRC: a modified CD13/APN peptidic homing motif.

2. Analysis of cell surface molecular distributions and cellular signaling by flow cytometry.

3. Fluorescence energy transfer as a probe for nucleic acid structures and sequences.

4. The X-ray crystal structure of human aminopeptidase N reveals a novel dimer and the basis for peptide processing.

5. Aminopeptidase N is a major receptor for the entero-pathogenic coronavirus TGEV.

6. Biogenetic pathways of plasma membrane proteins in Caco-2, a human intestinal epithelial cell line.

Review 7. The moonlighting enzyme CD13: old and new functions to target.