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-[[Image:1jn3.jpg|left|200px]]<br /><applet load="1jn3" size="450" color="white" frame="true" align="right" spinBox="true"
+[[Image:1jn3.jpg|left|200px]]<br /><applet load="1jn3" size="350" color="white" frame="true" align="right" spinBox="true"
 caption="1jn3, resolution 2.35&Aring;" />
 '''FIDELITY PROPERTIES AND STRUCTURE OF M282L MUTATOR MUTANT OF DNA POLYMERASE: SUBTLE STRUCTURAL CHANGES INFLUENCE THE MECHANISM OF NUCLEOTIDE DISCRIMINATION'''<br />
 ==Overview==
-DNA polymerase beta (pol beta) offers a simple system to examine the role, of polymerase structure in the fidelity of DNA synthesis. In this study, the M282L variant of pol beta (M282Lbeta) was identified using an in vivo, genetic screen. Met282, which does not contact the DNA template or the, incoming deoxynucleoside triphosphate (dNTP) substrate, is located on, alpha-helix N of pol beta. This mutant enzyme demonstrates increased, mutagenesis in both in vivo and in vitro assays. M282Lbeta has a 7.5-fold, higher mutation frequency than wild-type pol beta; M282Lbeta commits a, variety of base substitution and frameshift errors. Transient-state, kinetic methods were used to investigate the mechanism of intrinsic, mutator activity of M282Lbeta. Results show an 11-fold decrease in dNTP, substrate discrimination at the level of ground-state binding. However, during the protein conformational change and/or phosphodiester bond, formation, the nucleotide discrimination is improved. X-ray, crystallography was utilized to gain insights into the structural basis of, the decreased DNA synthesis fidelity. Most of the structural changes are, localized to site 282 and the surrounding region in the C-terminal part of, the 31-kDa domain. Repositioning of mostly hydrophobic amino acid residues, in the core of the C-terminal portion generates a protein with enhanced, stability. The combination of structural and equilibrium unfolding data, suggests that the mechanism of nucleotide discrimination is possibly, affected by the compacting of the hydrophobic core around residue Leu282., Subsequent movement of an adjacent surface residue, Arg283, produces a, slight increase in volume of the pocket that may accommodate the incoming, correct base pair. The structural changes of M282Lbeta ultimately lead to, an overall reduction in polymerase fidelity.
+DNA polymerase beta (pol beta) offers a simple system to examine the role of polymerase structure in the fidelity of DNA synthesis. In this study, the M282L variant of pol beta (M282Lbeta) was identified using an in vivo genetic screen. Met282, which does not contact the DNA template or the incoming deoxynucleoside triphosphate (dNTP) substrate, is located on alpha-helix N of pol beta. This mutant enzyme demonstrates increased mutagenesis in both in vivo and in vitro assays. M282Lbeta has a 7.5-fold higher mutation frequency than wild-type pol beta; M282Lbeta commits a variety of base substitution and frameshift errors. Transient-state kinetic methods were used to investigate the mechanism of intrinsic mutator activity of M282Lbeta. Results show an 11-fold decrease in dNTP substrate discrimination at the level of ground-state binding. However, during the protein conformational change and/or phosphodiester bond formation, the nucleotide discrimination is improved. X-ray crystallography was utilized to gain insights into the structural basis of the decreased DNA synthesis fidelity. Most of the structural changes are localized to site 282 and the surrounding region in the C-terminal part of the 31-kDa domain. Repositioning of mostly hydrophobic amino acid residues in the core of the C-terminal portion generates a protein with enhanced stability. The combination of structural and equilibrium unfolding data suggests that the mechanism of nucleotide discrimination is possibly affected by the compacting of the hydrophobic core around residue Leu282. Subsequent movement of an adjacent surface residue, Arg283, produces a slight increase in volume of the pocket that may accommodate the incoming correct base pair. The structural changes of M282Lbeta ultimately lead to an overall reduction in polymerase fidelity.
 ==About this Structure==
-JN3 is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Rattus_norvegicus Rattus norvegicus]. Active as [http://en.wikipedia.org/wiki/DNA-directed_DNA_polymerase DNA-directed DNA polymerase], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=2.7.7.7 2.7.7.7] Full crystallographic information is available from [http://ispc.weizmann.ac.il/oca-bin/ocashort?id=1JN3 OCA].
+JN3 is a [http://en.wikipedia.org/wiki/Single_protein Single protein] structure of sequence from [http://en.wikipedia.org/wiki/Rattus_norvegicus Rattus norvegicus]. Active as [http://en.wikipedia.org/wiki/DNA-directed_DNA_polymerase DNA-directed DNA polymerase], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=2.7.7.7 2.7.7.7] Full crystallographic information is available from [http://oca.weizmann.ac.il/oca-bin/ocashort?id=1JN3 OCA].
 ==Reference==
@@ Line 14: / Line 14: @@
 [[Category: Rattus norvegicus]]
 [[Category: Single protein]]
-[[Category: Conn, D.A.]]
+[[Category: Conn, D A.]]
 [[Category: Jaeger, J.]]
-[[Category: Sweasy, J.B.]]
+[[Category: Sweasy, J B.]]
 [[Category: dna polymerase beta (fragment)]]
 [[Category: mutant]]
 [[Category: nucleotide discrimination]]
-''Page seeded by [http://ispc.weizmann.ac.il/oca OCA ] on Tue Nov 20 18:23:48 2007''
+''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 13:24:27 2008''