Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin

Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin

Two alternative T7 RNA promoter/polymerase systems have been employed for the heterologous expression of a plant-type [2Fe-2S]ferredoxin, Anabaena 7120 vegetative ferredoxin, in Escherichia coli at high levels (∼20 mg/liter of culture). One system was used when 15N-labeling the ferredoxin uniformly...

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Veröffentlicht in:Archives of biochemistry and biophysics 1995-01, Vol.316 (1), p.619-634
Hauptverfasser: Cheng, H., Westler, W.M., Xia, B., Oh, B.H., Markley, J.L.
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Sprache:eng
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ANABAENA
Anabaena - chemistry
Anabaena - genetics
Arginine - chemistry
AZUFRE
Bacterial Proteins - biosynthesis
Bacterial Proteins - chemistry
Bacterial Proteins - genetics
Base Sequence
Carbon Isotopes
Carrier Proteins
CISTEINA
CLONACION
CLONAGE
CYSTEINE
Cysteine - chemistry
Deuterium
ESCHERICHIA COLI
ESPECTROMETRIA
EXPRESION GENICA
EXPRESSION DES GENES
FER
Ferredoxins - biosynthesis
Ferredoxins - chemistry
Ferredoxins - genetics
HIERRO
Isotope Labeling
Ligands
Magnetic Resonance Spectroscopy
METALLOPROTEINE
METALPROTEINAS
Molecular Sequence Data
Nitrogen Isotopes
PROTEINAS
PROTEINE
Recombinant Proteins - biosynthesis
Recombinant Proteins - chemistry
SOUFRE
SPECTROMETRIE
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Westler, W.M.
Xia, B.
Oh, B.H.
Markley, J.L.
description Two alternative T7 RNA promoter/polymerase systems have been employed for the heterologous expression of a plant-type [2Fe-2S]ferredoxin, Anabaena 7120 vegetative ferredoxin, in Escherichia coli at high levels (∼20 mg/liter of culture). One system was used when 15N-labeling the ferredoxin uniformly by growing E. coli with 15NH4Cl as the nitrogen source; the other was used in conjunction with auxotrophic host strains to enrich the protein selectively by incorporating 2H-, 13C-, and 15N-labeled amino acids. The labeled ferredoxin samples were studied by 1H, 2H, 13C and 15N NMR spectroscopy. Results from 1H and 2H NMR studies of samples containing [2Hα]Cys, [2Hβ2,β3]Cys, [13Cβ]-Cys, and [15N]Cys have confirmed previous cysteinyl proton resonance assignments (L. Skjeldal, W. M. Westler, B.-H. Oh, A. M. Krezel, H. M., Holden, B. L. Jacobson, I. Rayment, and J. L. Markley (1991) Biochemistry 30, 7363-7368). All four 13C NMR peaks arising from the four cysteinyl β-carbons and all four 15N NMR peaks from the four cysteinyl nitrogens were resolved in spectra of both the oxidized and reduced ferredoxins. The nitrogen resonance of Cys46, which is located in a unique (Ala-Cys) dipeptide, was assigned by detection of 13Ci-15Ni+1 coupling in a ferredoxin sample with incorporated [13C′]Ala and [15N]Cys. The nitrogen signal of Cys41 was assigned tentatively on the basis of its chemical shift and T1 relaxation time. The cysteinyl β-carbon resonances in the reduced state have been assigned to individual residues on the basis of correlations with their (previously assigned) β-protons. The β-carbon resonance from Cys46 in the oxidized state has been assigned by its correlation with the corresponding resonance in the reduced state; this was accomplished by following the progressive air oxidation of a protein sample reduced by dithionite in the presence of methyl viologen. The spin-lattice relaxation times of the β-carbons of the two cysteines coordinated to Fe(III) were similar in the oxidized and reduced states. This suggests that the antiferromagnetic coupling present in the reduced cluster has little influence on the electronic relaxation time of the Fe(III). Studies of the temperature dependence of the 1H, 13C, and 15N signals of the cysteinyl ligands to the [2Fe-2S] cluster show that the slope of the temperature dependence (Δδ/ΔT−1) can be different for different atom types within a given residue. For example, in the reduced ferredoxin, although Δδ/ΔT−1 is positive for Cy
doi_str_mv 10.1006/abbi.1995.1082
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One system was used when 15N-labeling the ferredoxin uniformly by growing E. coli with 15NH4Cl as the nitrogen source; the other was used in conjunction with auxotrophic host strains to enrich the protein selectively by incorporating 2H-, 13C-, and 15N-labeled amino acids. The labeled ferredoxin samples were studied by 1H, 2H, 13C and 15N NMR spectroscopy. Results from 1H and 2H NMR studies of samples containing [2Hα]Cys, [2Hβ2,β3]Cys, [13Cβ]-Cys, and [15N]Cys have confirmed previous cysteinyl proton resonance assignments (L. Skjeldal, W. M. Westler, B.-H. Oh, A. M. Krezel, H. M., Holden, B. L. Jacobson, I. Rayment, and J. L. Markley (1991) Biochemistry 30, 7363-7368). All four 13C NMR peaks arising from the four cysteinyl β-carbons and all four 15N NMR peaks from the four cysteinyl nitrogens were resolved in spectra of both the oxidized and reduced ferredoxins. The nitrogen resonance of Cys46, which is located in a unique (Ala-Cys) dipeptide, was assigned by detection of 13Ci-15Ni+1 coupling in a ferredoxin sample with incorporated [13C′]Ala and [15N]Cys. The nitrogen signal of Cys41 was assigned tentatively on the basis of its chemical shift and T1 relaxation time. The cysteinyl β-carbon resonances in the reduced state have been assigned to individual residues on the basis of correlations with their (previously assigned) β-protons. The β-carbon resonance from Cys46 in the oxidized state has been assigned by its correlation with the corresponding resonance in the reduced state; this was accomplished by following the progressive air oxidation of a protein sample reduced by dithionite in the presence of methyl viologen. The spin-lattice relaxation times of the β-carbons of the two cysteines coordinated to Fe(III) were similar in the oxidized and reduced states. This suggests that the antiferromagnetic coupling present in the reduced cluster has little influence on the electronic relaxation time of the Fe(III). Studies of the temperature dependence of the 1H, 13C, and 15N signals of the cysteinyl ligands to the [2Fe-2S] cluster show that the slope of the temperature dependence (Δδ/ΔT−1) can be different for different atom types within a given residue. For example, in the reduced ferredoxin, although Δδ/ΔT−1 is positive for Cys491Hβ2 and 1Hβ3, it is negative for Cys4913Cβ. Although Δδ/ΔT−1 is negative for protons of cysteines ligated to Fe(II) and positive for protons of cysteines ligated to Fe(III), it is positive for all the cysteinyl nitrogens. Nearly complete assignments for the spin system of Arg42 were derived from NMR studies of three selectively labeled samples: ferredoxin incorporating [U-15N]Arg, [26% U-13C]Arg, and [2Hα,β2,β3]Arg. The resonance arising from the backbone amide nitrogen exhibited an unusual chemical shift at 201.6 ppm in the oxidized state but was unresolved in the reduced state. The NMR results indicate that the hydrogen bond observed between the Arg42 backbone nitrogen and a sulfide of the iron-sulfur cluster in the X-ray structure of the oxidized ferredoxin crystal (W. R. Rypniewski, W. R. Breiter, M. M. Benning, G. Wesenberg, B.-H. Oh, J. L. Markley, I. Rayment, and H. M. Holden (1991) Biochemistry 30, 4126-4131) is present in solution in both the oxidized and reduced forms of the protein. The results show that the noncysteinyl, hyperfine-shifted (peak "K") in the spectrum of the reduced ferredoxin does not arise from 1Hα of Arg42 as previously postulated.</description><identifier>ISSN: 0003-9861</identifier><identifier>EISSN: 1096-0384</identifier><identifier>DOI: 10.1006/abbi.1995.1082</identifier><identifier>PMID: 7840674</identifier><language>eng</language><publisher>United States: Elsevier Inc</publisher><subject>ANABAENA ; Anabaena - chemistry ; Anabaena - genetics ; Arginine - chemistry ; AZUFRE ; Bacterial Proteins - biosynthesis ; Bacterial Proteins - chemistry ; Bacterial Proteins - genetics ; Base Sequence ; Carbon Isotopes ; Carrier Proteins ; CISTEINA ; CLONACION ; CLONAGE ; CYSTEINE ; Cysteine - chemistry ; Deuterium ; ESCHERICHIA COLI ; ESPECTROMETRIA ; EXPRESION GENICA ; EXPRESSION DES GENES ; FER ; Ferredoxins - biosynthesis ; Ferredoxins - chemistry ; Ferredoxins - genetics ; HIERRO ; Isotope Labeling ; Ligands ; Magnetic Resonance Spectroscopy ; METALLOPROTEINE ; METALPROTEINAS ; Molecular Sequence Data ; Nitrogen Isotopes ; PROTEINAS ; PROTEINE ; Recombinant Proteins - biosynthesis ; Recombinant Proteins - chemistry ; SOUFRE ; SPECTROMETRIE</subject><ispartof>Archives of biochemistry and biophysics, 1995-01, Vol.316 (1), p.619-634</ispartof><rights>1995 Academic Press</rights><lds50>peer_reviewed</lds50><woscitedreferencessubscribed>false</woscitedreferencessubscribed><citedby>FETCH-LOGICAL-c358t-c62660ab06549cac87ee4e785af95d1a44cb075e6ee1845538151575250951523</citedby></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><linktohtml>$$Uhttps://dx.doi.org/10.1006/abbi.1995.1082$$EHTML$$P50$$Gelsevier$$H</linktohtml><link.rule.ids>314,777,781,3537,27905,27906,45976</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/7840674$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><creatorcontrib>Cheng, H.</creatorcontrib><creatorcontrib>Westler, W.M.</creatorcontrib><creatorcontrib>Xia, B.</creatorcontrib><creatorcontrib>Oh, B.H.</creatorcontrib><creatorcontrib>Markley, J.L.</creatorcontrib><title>Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin</title><title>Archives of biochemistry and biophysics</title><addtitle>Arch Biochem Biophys</addtitle><description>Two alternative T7 RNA promoter/polymerase systems have been employed for the heterologous expression of a plant-type [2Fe-2S]ferredoxin, Anabaena 7120 vegetative ferredoxin, in Escherichia coli at high levels (∼20 mg/liter of culture). One system was used when 15N-labeling the ferredoxin uniformly by growing E. coli with 15NH4Cl as the nitrogen source; the other was used in conjunction with auxotrophic host strains to enrich the protein selectively by incorporating 2H-, 13C-, and 15N-labeled amino acids. The labeled ferredoxin samples were studied by 1H, 2H, 13C and 15N NMR spectroscopy. Results from 1H and 2H NMR studies of samples containing [2Hα]Cys, [2Hβ2,β3]Cys, [13Cβ]-Cys, and [15N]Cys have confirmed previous cysteinyl proton resonance assignments (L. Skjeldal, W. M. Westler, B.-H. Oh, A. M. Krezel, H. M., Holden, B. L. Jacobson, I. Rayment, and J. L. Markley (1991) Biochemistry 30, 7363-7368). All four 13C NMR peaks arising from the four cysteinyl β-carbons and all four 15N NMR peaks from the four cysteinyl nitrogens were resolved in spectra of both the oxidized and reduced ferredoxins. The nitrogen resonance of Cys46, which is located in a unique (Ala-Cys) dipeptide, was assigned by detection of 13Ci-15Ni+1 coupling in a ferredoxin sample with incorporated [13C′]Ala and [15N]Cys. The nitrogen signal of Cys41 was assigned tentatively on the basis of its chemical shift and T1 relaxation time. The cysteinyl β-carbon resonances in the reduced state have been assigned to individual residues on the basis of correlations with their (previously assigned) β-protons. The β-carbon resonance from Cys46 in the oxidized state has been assigned by its correlation with the corresponding resonance in the reduced state; this was accomplished by following the progressive air oxidation of a protein sample reduced by dithionite in the presence of methyl viologen. The spin-lattice relaxation times of the β-carbons of the two cysteines coordinated to Fe(III) were similar in the oxidized and reduced states. This suggests that the antiferromagnetic coupling present in the reduced cluster has little influence on the electronic relaxation time of the Fe(III). Studies of the temperature dependence of the 1H, 13C, and 15N signals of the cysteinyl ligands to the [2Fe-2S] cluster show that the slope of the temperature dependence (Δδ/ΔT−1) can be different for different atom types within a given residue. For example, in the reduced ferredoxin, although Δδ/ΔT−1 is positive for Cys491Hβ2 and 1Hβ3, it is negative for Cys4913Cβ. Although Δδ/ΔT−1 is negative for protons of cysteines ligated to Fe(II) and positive for protons of cysteines ligated to Fe(III), it is positive for all the cysteinyl nitrogens. Nearly complete assignments for the spin system of Arg42 were derived from NMR studies of three selectively labeled samples: ferredoxin incorporating [U-15N]Arg, [26% U-13C]Arg, and [2Hα,β2,β3]Arg. The resonance arising from the backbone amide nitrogen exhibited an unusual chemical shift at 201.6 ppm in the oxidized state but was unresolved in the reduced state. The NMR results indicate that the hydrogen bond observed between the Arg42 backbone nitrogen and a sulfide of the iron-sulfur cluster in the X-ray structure of the oxidized ferredoxin crystal (W. R. Rypniewski, W. R. Breiter, M. M. Benning, G. Wesenberg, B.-H. Oh, J. L. Markley, I. Rayment, and H. M. Holden (1991) Biochemistry 30, 4126-4131) is present in solution in both the oxidized and reduced forms of the protein. The results show that the noncysteinyl, hyperfine-shifted (peak "K") in the spectrum of the reduced ferredoxin does not arise from 1Hα of Arg42 as previously postulated.</description><subject>ANABAENA</subject><subject>Anabaena - chemistry</subject><subject>Anabaena - genetics</subject><subject>Arginine - chemistry</subject><subject>AZUFRE</subject><subject>Bacterial Proteins - biosynthesis</subject><subject>Bacterial Proteins - chemistry</subject><subject>Bacterial Proteins - genetics</subject><subject>Base Sequence</subject><subject>Carbon Isotopes</subject><subject>Carrier Proteins</subject><subject>CISTEINA</subject><subject>CLONACION</subject><subject>CLONAGE</subject><subject>CYSTEINE</subject><subject>Cysteine - chemistry</subject><subject>Deuterium</subject><subject>ESCHERICHIA COLI</subject><subject>ESPECTROMETRIA</subject><subject>EXPRESION GENICA</subject><subject>EXPRESSION DES GENES</subject><subject>FER</subject><subject>Ferredoxins - biosynthesis</subject><subject>Ferredoxins - chemistry</subject><subject>Ferredoxins - genetics</subject><subject>HIERRO</subject><subject>Isotope Labeling</subject><subject>Ligands</subject><subject>Magnetic Resonance Spectroscopy</subject><subject>METALLOPROTEINE</subject><subject>METALPROTEINAS</subject><subject>Molecular Sequence Data</subject><subject>Nitrogen Isotopes</subject><subject>PROTEINAS</subject><subject>PROTEINE</subject><subject>Recombinant Proteins - biosynthesis</subject><subject>Recombinant Proteins - chemistry</subject><subject>SOUFRE</subject><subject>SPECTROMETRIE</subject><issn>0003-9861</issn><issn>1096-0384</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>1995</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNp1kUFv1DAQhS1EVZaWKwckJJ84NYud2I59rKourbQtiLRcELIcZ7IYZe3UzlbdH8F_rre74sbJY71v3thvEHpPyZwSIj6btnVzqhTPV1m-QjNKlChIJdlrNCOEVIWSgr5Bb1P6QwilTJTH6LiWjIiazdDfbzFM4Dy-fBojpOSCP8MNDGAn9wj4OoUpjM7ipWlhcH51ho3v8Lk3wza5hEOPr7YjxN55KJrfrp-gw7c333HjVpl5ATLcGvAG17Qk-AesYDIv5j_LBRRl82sBMUIXnpw_RUd97oJ3h_ME3S8u7y6uiuXXL9cX58vCVlxOhRWlEMS0RHCmrLGyBmBQS256xTtqGLMtqTkIACoZ55WknPKal5yoXJTVCfq09x1jeNhAmvTaJQvDYDyETdJ1fqqSlGVwvgdtDClF6PUY3drEraZE7_LXu_z1Ln-9yz83fDw4b9o1dP_wQ-BZ_7DXexO0WUWX9H2jOOOSVFmUexHy3x8dRJ2sA2-hczEvRHfB_W_uM0vJm14</recordid><startdate>19950110</startdate><enddate>19950110</enddate><creator>Cheng, H.</creator><creator>Westler, W.M.</creator><creator>Xia, B.</creator><creator>Oh, B.H.</creator><creator>Markley, J.L.</creator><general>Elsevier Inc</general><scope>FBQ</scope><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7X8</scope></search><sort><creationdate>19950110</creationdate><title>Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin</title><author>Cheng, H. ; Westler, W.M. ; Xia, B. ; Oh, B.H. ; Markley, J.L.</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c358t-c62660ab06549cac87ee4e785af95d1a44cb075e6ee1845538151575250951523</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>1995</creationdate><topic>ANABAENA</topic><topic>Anabaena - chemistry</topic><topic>Anabaena - genetics</topic><topic>Arginine - chemistry</topic><topic>AZUFRE</topic><topic>Bacterial Proteins - biosynthesis</topic><topic>Bacterial Proteins - chemistry</topic><topic>Bacterial Proteins - genetics</topic><topic>Base Sequence</topic><topic>Carbon Isotopes</topic><topic>Carrier Proteins</topic><topic>CISTEINA</topic><topic>CLONACION</topic><topic>CLONAGE</topic><topic>CYSTEINE</topic><topic>Cysteine - chemistry</topic><topic>Deuterium</topic><topic>ESCHERICHIA COLI</topic><topic>ESPECTROMETRIA</topic><topic>EXPRESION GENICA</topic><topic>EXPRESSION DES GENES</topic><topic>FER</topic><topic>Ferredoxins - biosynthesis</topic><topic>Ferredoxins - chemistry</topic><topic>Ferredoxins - genetics</topic><topic>HIERRO</topic><topic>Isotope Labeling</topic><topic>Ligands</topic><topic>Magnetic Resonance Spectroscopy</topic><topic>METALLOPROTEINE</topic><topic>METALPROTEINAS</topic><topic>Molecular Sequence Data</topic><topic>Nitrogen Isotopes</topic><topic>PROTEINAS</topic><topic>PROTEINE</topic><topic>Recombinant Proteins - biosynthesis</topic><topic>Recombinant Proteins - chemistry</topic><topic>SOUFRE</topic><topic>SPECTROMETRIE</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Cheng, H.</creatorcontrib><creatorcontrib>Westler, W.M.</creatorcontrib><creatorcontrib>Xia, B.</creatorcontrib><creatorcontrib>Oh, B.H.</creatorcontrib><creatorcontrib>Markley, J.L.</creatorcontrib><collection>AGRIS</collection><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>MEDLINE - Academic</collection><jtitle>Archives of biochemistry and biophysics</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Cheng, H.</au><au>Westler, W.M.</au><au>Xia, B.</au><au>Oh, B.H.</au><au>Markley, J.L.</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin</atitle><jtitle>Archives of biochemistry and biophysics</jtitle><addtitle>Arch Biochem Biophys</addtitle><date>1995-01-10</date><risdate>1995</risdate><volume>316</volume><issue>1</issue><spage>619</spage><epage>634</epage><pages>619-634</pages><issn>0003-9861</issn><eissn>1096-0384</eissn><abstract>Two alternative T7 RNA promoter/polymerase systems have been employed for the heterologous expression of a plant-type [2Fe-2S]ferredoxin, Anabaena 7120 vegetative ferredoxin, in Escherichia coli at high levels (∼20 mg/liter of culture). One system was used when 15N-labeling the ferredoxin uniformly by growing E. coli with 15NH4Cl as the nitrogen source; the other was used in conjunction with auxotrophic host strains to enrich the protein selectively by incorporating 2H-, 13C-, and 15N-labeled amino acids. The labeled ferredoxin samples were studied by 1H, 2H, 13C and 15N NMR spectroscopy. Results from 1H and 2H NMR studies of samples containing [2Hα]Cys, [2Hβ2,β3]Cys, [13Cβ]-Cys, and [15N]Cys have confirmed previous cysteinyl proton resonance assignments (L. Skjeldal, W. M. Westler, B.-H. Oh, A. M. Krezel, H. M., Holden, B. L. Jacobson, I. Rayment, and J. L. Markley (1991) Biochemistry 30, 7363-7368). All four 13C NMR peaks arising from the four cysteinyl β-carbons and all four 15N NMR peaks from the four cysteinyl nitrogens were resolved in spectra of both the oxidized and reduced ferredoxins. The nitrogen resonance of Cys46, which is located in a unique (Ala-Cys) dipeptide, was assigned by detection of 13Ci-15Ni+1 coupling in a ferredoxin sample with incorporated [13C′]Ala and [15N]Cys. The nitrogen signal of Cys41 was assigned tentatively on the basis of its chemical shift and T1 relaxation time. The cysteinyl β-carbon resonances in the reduced state have been assigned to individual residues on the basis of correlations with their (previously assigned) β-protons. The β-carbon resonance from Cys46 in the oxidized state has been assigned by its correlation with the corresponding resonance in the reduced state; this was accomplished by following the progressive air oxidation of a protein sample reduced by dithionite in the presence of methyl viologen. The spin-lattice relaxation times of the β-carbons of the two cysteines coordinated to Fe(III) were similar in the oxidized and reduced states. This suggests that the antiferromagnetic coupling present in the reduced cluster has little influence on the electronic relaxation time of the Fe(III). Studies of the temperature dependence of the 1H, 13C, and 15N signals of the cysteinyl ligands to the [2Fe-2S] cluster show that the slope of the temperature dependence (Δδ/ΔT−1) can be different for different atom types within a given residue. For example, in the reduced ferredoxin, although Δδ/ΔT−1 is positive for Cys491Hβ2 and 1Hβ3, it is negative for Cys4913Cβ. Although Δδ/ΔT−1 is negative for protons of cysteines ligated to Fe(II) and positive for protons of cysteines ligated to Fe(III), it is positive for all the cysteinyl nitrogens. Nearly complete assignments for the spin system of Arg42 were derived from NMR studies of three selectively labeled samples: ferredoxin incorporating [U-15N]Arg, [26% U-13C]Arg, and [2Hα,β2,β3]Arg. The resonance arising from the backbone amide nitrogen exhibited an unusual chemical shift at 201.6 ppm in the oxidized state but was unresolved in the reduced state. The NMR results indicate that the hydrogen bond observed between the Arg42 backbone nitrogen and a sulfide of the iron-sulfur cluster in the X-ray structure of the oxidized ferredoxin crystal (W. R. Rypniewski, W. R. Breiter, M. M. Benning, G. Wesenberg, B.-H. Oh, J. L. Markley, I. Rayment, and H. M. Holden (1991) Biochemistry 30, 4126-4131) is present in solution in both the oxidized and reduced forms of the protein. The results show that the noncysteinyl, hyperfine-shifted (peak "K") in the spectrum of the reduced ferredoxin does not arise from 1Hα of Arg42 as previously postulated.</abstract><cop>United States</cop><pub>Elsevier Inc</pub><pmid>7840674</pmid><doi>10.1006/abbi.1995.1082</doi><tpages>16</tpages></addata></record>
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identifier ISSN: 0003-9861
ispartof Archives of biochemistry and biophysics, 1995-01, Vol.316 (1), p.619-634
issn 0003-9861
1096-0384
language eng
recordid cdi_proquest_miscellaneous_77129814
source MEDLINE; Elsevier ScienceDirect Journals
subjects ANABAENA
Anabaena - chemistry
Anabaena - genetics
Arginine - chemistry
AZUFRE
Bacterial Proteins - biosynthesis
Bacterial Proteins - chemistry
Bacterial Proteins - genetics
Base Sequence
Carbon Isotopes
Carrier Proteins
CISTEINA
CLONACION
CLONAGE
CYSTEINE
Cysteine - chemistry
Deuterium
ESCHERICHIA COLI
ESPECTROMETRIA
EXPRESION GENICA
EXPRESSION DES GENES
FER
Ferredoxins - biosynthesis
Ferredoxins - chemistry
Ferredoxins - genetics
HIERRO
Isotope Labeling
Ligands
Magnetic Resonance Spectroscopy
METALLOPROTEINE
METALPROTEINAS
Molecular Sequence Data
Nitrogen Isotopes
PROTEINAS
PROTEINE
Recombinant Proteins - biosynthesis
Recombinant Proteins - chemistry
SOUFRE
SPECTROMETRIE
title Protein Expression, Selective Isotopic Labeling, and Analysis of Hyperfine-Shifted NMR Signals of Anabaena 7120 Vegetative [2Fe-2S]Ferredoxin
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