Literature DB >> 12846839

Structure and positioning comparison of two variants of penetratin in two different membrane mimicking systems by NMR.

Mattias Lindberg1, Henrik Biverståhl, Astrid Gräslund, Lena Mäler.   

Abstract

The Antennapedia homeodomain protein of Drosophila has the ability to penetrate biological membranes and the third helix of this protein, residues 43-58, known as penetratin (RQIKIWFQNRRMKWKK-amide) has the same translocating properties as the entire protein. The variant, RQI KIFFQNRRMKFKK-amide, here called penetratin (W48F,W56F) does not have the same ability. We have determined a solution structure of penetratin and investigated the position of both peptides in negatively charged bicelles. A helical structure is seen for residues Lys46 through Met54. The secondary structure of the variant penetratin(W48F,W56F) in bicelles appears to be very similar. Paramagnetic spin-label studies and analysis of NOEs between penetratin and the phospholipids show that penetratin is located within the bicelle surface. Penetratin (W48F,W56F) is also located inside the phospholipid bicelle, however, with its N-terminus more deeply inserted than that of wild-type penetratin. The subtle differences in the way the two peptides interact with a membrane in an equilibrium situation could be important for their translocating ability. As a comparison we have also investigated the secondary structure of penetratin(W48F,W56F) in SDS micelles and the results show that the structure is very similar in SDS and bicelles. In contrast, penetratin(W48F,W56F) and penetratin appear to be located differently in SDS micelles. This clearly shows the importance of using realistic membrane mimetics for investigating peptide-membrane interactions.

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Year:  2003        PMID: 12846839     DOI: 10.1046/j.1432-1033.2003.03685.x

Source DB:  PubMed          Journal:  Eur J Biochem        ISSN: 0014-2956


  23 in total

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5.  Structure and dynamics of cationic membrane peptides and proteins: insights from solid-state NMR.

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7.  Membrane surface-associated helices promote lipid interactions and cellular uptake of human calcitonin-derived cell penetrating peptides.

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8.  Structural characterization of AS1-membrane interactions from a subset of HAMP domains.

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9.  Relative free energy of binding between antimicrobial peptides and SDS or DPC micelles.

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10.  Determination of penetratin secondary structure in live cells with Raman microscopy.

Authors:  Jing Ye; Sara A Fox; Mare Cudic; Evonne M Rezler; Janelle L Lauer; Gregg B Fields; Andrew C Terentis
Journal:  J Am Chem Soc       Date:  2010-01-27       Impact factor: 15.419

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