1fp4

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Revision as of 10:41, 21 February 2008

CRYSTAL STRUCTURE OF THE ALPHA-H195Q MUTANT OF NITROGENASE

Overview

EPR signals observed under CO and C(2)H(2) during nitrogenase turnover were investigated for the alpha-Gln(195) MoFe protein, an altered form for which the alpha-His(195) residue has been substituted by glutamine. Under CO, samples show S = 1/2 hi- and lo-CO EPR signals identical to those recognized for the wild-type protein, whereas the S = 3/2 signals generated under high CO/high flux conditions differ. Previous work has revealed that the EPR spectrum generated under C(2)H(2) exhibits a signal (S(EPR1)) originating from the FeMo-cofactor having two or more bound C(2)H(2) adducts and a second signal (S(EPR2)) arising from a radical species [Sorlie, M., Christiansen, J., Dean, D. R., and Hales, B. J. (1999) J. Am. Chem. Soc. 121, 9457-9458]. Pressure-dependent studies show that the intensity of these signals has a sigmoidal dependency at low pressures and maximized at 0.1 atm C(2)H(2) with a subsequent decrease in steady-state intensity at higher pressures. Analogous signals are not recognized for the wild-type MoFe protein. Analysis of the principal g-factors of S(EPR2) suggests that it either represents an unusual metal cluster or is a carboxylate centered radical possibly originating from homocitrate. Both S(EPR1) and S(EPR2) exhibit similar relaxation properties that are atypical for S = 1/2 signals originating from Fe-S clusters or radicals and indicate a coupled relaxation pathway. The alpha-Gln(195) MoFe protein also exhibits these signals when incubated under turnover conditions in the presence of C(2)H(4). Under these conditions, additional inflections in the g 4-6 region assigned to ground-state transitions of an S = 3/2 spin system are also recognized and assigned to turnover states of the MoFe protein without C(2)H(4) bound. The structure of alpha-Gln(195) was crystallographically determined and found to be virtually identical to that of the wild-type MoFe protein except for replacement of an NuH-S hydrogen bond interaction between FeMo-cofactor and the imidazole side chain of alpha-His(195) by an analogous interaction involving Gln.

About this Structure

1FP4 is a Protein complex structure of sequences from Azotobacter vinelandii with , , and as ligands. Active as Nitrogenase, with EC number 1.18.6.1 Full crystallographic information is available from OCA.

Reference

Mechanistic features and structure of the nitrogenase alpha-Gln195 MoFe protein., Sorlie M, Christiansen J, Lemon BJ, Peters JW, Dean DR, Hales BJ, Biochemistry. 2001 Feb 13;40(6):1540-9. PMID:11327812

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Retrieved from "http://52.214.119.220/wiki/index.php/1fp4"

@@ Line 1: / Line 1: @@
-[[Image:1fp4.jpg|left|200px]]<br /><applet load="1fp4" size="450" color="white" frame="true" align="right" spinBox="true"
+[[Image:1fp4.jpg|left|200px]]<br /><applet load="1fp4" size="350" color="white" frame="true" align="right" spinBox="true"
 caption="1fp4, resolution 2.5&Aring;" />
 '''CRYSTAL STRUCTURE OF THE ALPHA-H195Q MUTANT OF NITROGENASE'''<br />
 ==Overview==
-EPR signals observed under CO and C(2)H(2) during nitrogenase turnover, were investigated for the alpha-Gln(195) MoFe protein, an altered form for, which the alpha-His(195) residue has been substituted by glutamine. Under, CO, samples show S = 1/2 hi- and lo-CO EPR signals identical to those, recognized for the wild-type protein, whereas the S = 3/2 signals, generated under high CO/high flux conditions differ. Previous work has, revealed that the EPR spectrum generated under C(2)H(2) exhibits a signal, (S(EPR1)) originating from the FeMo-cofactor having two or more bound, C(2)H(2) adducts and a second signal (S(EPR2)) arising from a radical, species [Sorlie, M., Christiansen, J., Dean, D. R., and Hales, B. J., (1999) J. Am. Chem. Soc. 121, 9457-9458]. Pressure-dependent studies show, that the intensity of these signals has a sigmoidal dependency at low, pressures and maximized at 0.1 atm C(2)H(2) with a subsequent decrease in, steady-state intensity at higher pressures. Analogous signals are not, recognized for the wild-type MoFe protein. Analysis of the principal, g-factors of S(EPR2) suggests that it either represents an unusual metal, cluster or is a carboxylate centered radical possibly originating from, homocitrate. Both S(EPR1) and S(EPR2) exhibit similar relaxation, properties that are atypical for S = 1/2 signals originating from Fe-S, clusters or radicals and indicate a coupled relaxation pathway. The, alpha-Gln(195) MoFe protein also exhibits these signals when incubated, under turnover conditions in the presence of C(2)H(4). Under these, conditions, additional inflections in the g 4-6 region assigned to, ground-state transitions of an S = 3/2 spin system are also recognized and, assigned to turnover states of the MoFe protein without C(2)H(4) bound., The structure of alpha-Gln(195) was crystallographically determined and, found to be virtually identical to that of the wild-type MoFe protein, except for replacement of an NuH-S hydrogen bond interaction between, FeMo-cofactor and the imidazole side chain of alpha-His(195) by an, analogous interaction involving Gln.
+EPR signals observed under CO and C(2)H(2) during nitrogenase turnover were investigated for the alpha-Gln(195) MoFe protein, an altered form for which the alpha-His(195) residue has been substituted by glutamine. Under CO, samples show S = 1/2 hi- and lo-CO EPR signals identical to those recognized for the wild-type protein, whereas the S = 3/2 signals generated under high CO/high flux conditions differ. Previous work has revealed that the EPR spectrum generated under C(2)H(2) exhibits a signal (S(EPR1)) originating from the FeMo-cofactor having two or more bound C(2)H(2) adducts and a second signal (S(EPR2)) arising from a radical species [Sorlie, M., Christiansen, J., Dean, D. R., and Hales, B. J. (1999) J. Am. Chem. Soc. 121, 9457-9458]. Pressure-dependent studies show that the intensity of these signals has a sigmoidal dependency at low pressures and maximized at 0.1 atm C(2)H(2) with a subsequent decrease in steady-state intensity at higher pressures. Analogous signals are not recognized for the wild-type MoFe protein. Analysis of the principal g-factors of S(EPR2) suggests that it either represents an unusual metal cluster or is a carboxylate centered radical possibly originating from homocitrate. Both S(EPR1) and S(EPR2) exhibit similar relaxation properties that are atypical for S = 1/2 signals originating from Fe-S clusters or radicals and indicate a coupled relaxation pathway. The alpha-Gln(195) MoFe protein also exhibits these signals when incubated under turnover conditions in the presence of C(2)H(4). Under these conditions, additional inflections in the g 4-6 region assigned to ground-state transitions of an S = 3/2 spin system are also recognized and assigned to turnover states of the MoFe protein without C(2)H(4) bound. The structure of alpha-Gln(195) was crystallographically determined and found to be virtually identical to that of the wild-type MoFe protein except for replacement of an NuH-S hydrogen bond interaction between FeMo-cofactor and the imidazole side chain of alpha-His(195) by an analogous interaction involving Gln.
 ==About this Structure==
-FP4 is a [http://en.wikipedia.org/wiki/Protein_complex Protein complex] structure of sequences from [http://en.wikipedia.org/wiki/Azotobacter_vinelandii Azotobacter vinelandii] with CA, HCA, CFM and CLP as [http://en.wikipedia.org/wiki/ligands ligands]. Active as [http://en.wikipedia.org/wiki/Nitrogenase Nitrogenase], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=1.18.6.1 1.18.6.1] Full crystallographic information is available from [http://ispc.weizmann.ac.il/oca-bin/ocashort?id=1FP4 OCA].
+FP4 is a [http://en.wikipedia.org/wiki/Protein_complex Protein complex] structure of sequences from [http://en.wikipedia.org/wiki/Azotobacter_vinelandii Azotobacter vinelandii] with <scene name='pdbligand=CA:'>CA</scene>, <scene name='pdbligand=HCA:'>HCA</scene>, <scene name='pdbligand=CFM:'>CFM</scene> and <scene name='pdbligand=CLP:'>CLP</scene> as [http://en.wikipedia.org/wiki/ligands ligands]. Active as [http://en.wikipedia.org/wiki/Nitrogenase Nitrogenase], with EC number [http://www.brenda-enzymes.info/php/result_flat.php4?ecno=1.18.6.1 1.18.6.1] Full crystallographic information is available from [http://oca.weizmann.ac.il/oca-bin/ocashort?id=1FP4 OCA].
 ==Reference==
@@ Line 15: / Line 15: @@
 [[Category: Protein complex]]
 [[Category: Christiansen, J.]]
-[[Category: Dean, D.R.]]
+[[Category: Dean, D R.]]
-[[Category: Hales, B.J.]]
+[[Category: Hales, B J.]]
-[[Category: Lemon, B.J.]]
+[[Category: Lemon, B J.]]
-[[Category: Peters, J.W.]]
+[[Category: Peters, J W.]]
 [[Category: Sorlie, M.]]
 [[Category: CA]]
@@ Line 26: / Line 26: @@
 [[Category: iron-sulfur-molybdenum protein]]
-''Page seeded by [http://ispc.weizmann.ac.il/oca OCA ] on Tue Nov 20 15:06:41 2007''
+''Page seeded by [http://oca.weizmann.ac.il/oca OCA ] on Thu Feb 21 12:41:03 2008''

1fp4

From Proteopedia

Revision as of 10:41, 21 February 2008

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