1llt

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(New page: 200px<br /> <applet load="1llt" size="450" color="white" frame="true" align="right" spinBox="true" caption="1llt, resolution 3.10&Aring;" /> '''BIRCH POLLEN ALLERG...)
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'''BIRCH POLLEN ALLERGEN BET V 1 MUTANT E45S'''<br />
'''BIRCH POLLEN ALLERGEN BET V 1 MUTANT E45S'''<br />
==Overview==
==Overview==
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Specific allergy vaccination is an efficient treatment for allergic, disease; however, the development of safer vaccines would enable a more, general use of the treatment. Determination of molecular structures of, allergens and allergen-Ab complexes facilitates epitope mapping and, enables a rational approach to the engineering of allergen molecules with, reduced IgE binding. In this study, we describe the identification and, modification of a human IgE-binding epitope based on the crystal structure, of Bet v 1 in complex with the BV16 Fab' fragment. The epitope occupies, approximately 10% of the molecular surface area of Bet v 1 and is clearly, conformational. A synthetic peptide representing a sequential motif in the, epitope (11 of 16 residues) did not inhibit the binding of mAb BV16 to Bet, v 1, illustrating limitations in the use of peptides for B cell epitope, characterization. The single amino acid substitution, Glu(45)-Ser, was, introduced in the epitope and completely abolished the binding of mAb BV16, to the Bet v 1 mutant within a concentration range 1000-fold higher than, wild type. The mutant also showed up to 50% reduction in the binding of, human polyclonal IgE, demonstrating that glutamic acid 45 is a critical, amino acid also in a major human IgE-binding epitope. By solving the, three-dimensional crystal structure of the Bet v 1 Glu(45)-Ser mutant, it, was shown that the change in immunochemical activity is directly related, to the Glu(45)-Ser substitution and not to long-range structural, alterations or collapse of the Bet v 1 mutant tertiary structure.
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Specific allergy vaccination is an efficient treatment for allergic disease; however, the development of safer vaccines would enable a more general use of the treatment. Determination of molecular structures of allergens and allergen-Ab complexes facilitates epitope mapping and enables a rational approach to the engineering of allergen molecules with reduced IgE binding. In this study, we describe the identification and modification of a human IgE-binding epitope based on the crystal structure of Bet v 1 in complex with the BV16 Fab' fragment. The epitope occupies approximately 10% of the molecular surface area of Bet v 1 and is clearly conformational. A synthetic peptide representing a sequential motif in the epitope (11 of 16 residues) did not inhibit the binding of mAb BV16 to Bet v 1, illustrating limitations in the use of peptides for B cell epitope characterization. The single amino acid substitution, Glu(45)-Ser, was introduced in the epitope and completely abolished the binding of mAb BV16 to the Bet v 1 mutant within a concentration range 1000-fold higher than wild type. The mutant also showed up to 50% reduction in the binding of human polyclonal IgE, demonstrating that glutamic acid 45 is a critical amino acid also in a major human IgE-binding epitope. By solving the three-dimensional crystal structure of the Bet v 1 Glu(45)-Ser mutant, it was shown that the change in immunochemical activity is directly related to the Glu(45)-Ser substitution and not to long-range structural alterations or collapse of the Bet v 1 mutant tertiary structure.
==About this Structure==
==About this Structure==
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1LLT is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Betula_pendula Betula pendula]. Full crystallographic information is available from [http://ispc.weizmann.ac.il/oca-bin/ocashort?id=1LLT OCA].
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1LLT is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Betula_pendula Betula pendula]. Full crystallographic information is available from [http://oca.weizmann.ac.il/oca-bin/ocashort?id=1LLT OCA].
==Reference==
==Reference==
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[[Category: Gajhede, M.]]
[[Category: Gajhede, M.]]
[[Category: Ipsen, H.]]
[[Category: Ipsen, H.]]
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[[Category: Larsen, J.N.]]
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[[Category: Larsen, J N.]]
[[Category: Mirza, O.]]
[[Category: Mirza, O.]]
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[[Category: Neerven, R.J.Van.]]
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[[Category: Neerven, R J.Van.]]
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[[Category: Spangfort, M.D.]]
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[[Category: Spangfort, M D.]]
[[Category: allergen]]
[[Category: allergen]]
[[Category: pathogenesis related proteins]]
[[Category: pathogenesis related proteins]]
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''Page seeded by [http://ispc.weizmann.ac.il/oca OCA ] on Sun Nov 18 09:35:37 2007''
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''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 13:46:07 2008''

Revision as of 11:46, 21 February 2008

Image:1llt.gif

1llt, resolution 3.10Å

Drag the structure with the mouse to rotate

BIRCH POLLEN ALLERGEN BET V 1 MUTANT E45S

Overview

Specific allergy vaccination is an efficient treatment for allergic disease; however, the development of safer vaccines would enable a more general use of the treatment. Determination of molecular structures of allergens and allergen-Ab complexes facilitates epitope mapping and enables a rational approach to the engineering of allergen molecules with reduced IgE binding. In this study, we describe the identification and modification of a human IgE-binding epitope based on the crystal structure of Bet v 1 in complex with the BV16 Fab' fragment. The epitope occupies approximately 10% of the molecular surface area of Bet v 1 and is clearly conformational. A synthetic peptide representing a sequential motif in the epitope (11 of 16 residues) did not inhibit the binding of mAb BV16 to Bet v 1, illustrating limitations in the use of peptides for B cell epitope characterization. The single amino acid substitution, Glu(45)-Ser, was introduced in the epitope and completely abolished the binding of mAb BV16 to the Bet v 1 mutant within a concentration range 1000-fold higher than wild type. The mutant also showed up to 50% reduction in the binding of human polyclonal IgE, demonstrating that glutamic acid 45 is a critical amino acid also in a major human IgE-binding epitope. By solving the three-dimensional crystal structure of the Bet v 1 Glu(45)-Ser mutant, it was shown that the change in immunochemical activity is directly related to the Glu(45)-Ser substitution and not to long-range structural alterations or collapse of the Bet v 1 mutant tertiary structure.

About this Structure

1LLT is a Single protein structure of sequence from Betula pendula. Full crystallographic information is available from OCA.

Reference

Dominating IgE-binding epitope of Bet v 1, the major allergen of birch pollen, characterized by X-ray crystallography and site-directed mutagenesis., Spangfort MD, Mirza O, Ipsen H, Van Neerven RJ, Gajhede M, Larsen JN, J Immunol. 2003 Sep 15;171(6):3084-90. PMID:12960334

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