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VnfY Is Required for Full Activity of the Vanadium-Containing Dinitrogenase in Azotobacter vinelandii

Department of Biochemistry and Center for the Study of Nitrogen Fixation, College of Agricultural and Life Sciences, University of Wisconsin—Madison, Madison, Wisconsin 53706,¹ PanVera Corporation, Madison, Wisconsin ,² Department of Plant and Microbial Biology, University of California—Berkeley, Berkeley, California 94720,³ Department of Biochemistry, Virginia Polytechnic Institute and State University, Blacksburg, Virginia 24061-0346⁴

Received 1 July 2002/ Accepted 2 January 2003

	ABSTRACT

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A gene from Azotobacter vinelandii whose product exhibits primary sequence similarity to the NifY, NafY, NifX, and VnfX family of proteins, and which is required for effective V-dependent diazotrophic growth, was identified. Because this gene is located downstream from vnfK in an arrangement similar to the relative organization of the nifK and nifY genes, it was designated vnfY. A mutant strain having an insertion mutation in vnfY has 10-fold less vnf dinitrogenase activity and exhibits a greatly diminished level of ⁴⁹V label incorporation into the V-dependent dinitrogenase when compared to the wild type. These results indicate that VnfY has a role in the maturation of the V-dependent dinitrogenase, with a specific role in the formation of the V-containing cofactor and/or its insertion into apodinitrogenase.

	TEXT

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Azotobacter vinelandii harbors three genetically distinct nitrogenase systems that are differentially expressed depending on the availability of metals in the medium: a nif-encoded Mo-containing nitrogenase, a vnf-encoded V-containing nitrogenase, and an anf-encoded iron-only nitrogenase (2). The V-containing nitrogenase contains an iron-vanadium cofactor (FeV-co) at its active site which is structurally and functionally analogous to the better-characterized FeMo-co of the Mo-dependent system. A functional V-containing nitrogenase requires the products of the structural genes for dinitrogenase (vnfDGK) and dinitrogenase reductase (vnfH) as well as several other nif and vnf gene products involved in the biosynthesis of FeV-co and the maturation of the nitrogenase component proteins. Much of what is known about the biosynthesis of FeV-co comes from analogous studies on FeMo-co biosynthesis. It is believed that the products of nifB, vnfN, vnfE, vnfH, vnfX, and nifV are involved in the biosynthesis of FeV-co (see reference 12 for a review).

The involvement of VnfX in the biosynthesis of FeV-co is of particular interest with respect to the results described here. A vanadium-iron-sulfur cluster presumed to be similar to a precursor of FeMo-co biosynthesis accumulates on VnfX during FeV-co biosynthesis (16). Upon homocitrate addition, a newly formed homocitrate- and vanadium-containing cluster is transferred from VnfX to apodinitrogenase; the resulting dinitrogenase is able to reduce acetylene (15). VnfX is also able to bind structurally related metalloclusters as NifB-co or FeMo-co. The exact role of VnfX in FeV-co biosynthesis is not yet known.

To identify vnf genes whose products are involved in formation of a functional V-containing nitrogenase, we determined the nucleotide sequence of the genomic region located downstream from the previously characterized vnfDGK genes. This analysis revealed the presence of two open reading frames (ORFs) (Fig. 1). The sequence obtained in this work was also confirmed by comparison to the preliminary sequences provided by the shotgun sequence analysis of the entire A. vinelandii genome. The first ORF encodes a 161-residue polypeptide exhibiting primary sequence similarity to the VnfX, NifX, NifY, and NafY family of proteins. Because of these similarities and its chromosomal location relative to the structural genes for the vnf dinitrogenase, this potential gene was designated vnfY. The second ORF encodes the ATP-binding subunit of an ABC-type transporter of unknown function. The vnfY gene and ORF2 show a 3-bp overlap, indicating that their expression is tightly coupled.

View larger version (10K): [in this window] [in a new window]   FIG. 1. Structure of the A. vinelandii chromosome 3' of the vnfDGK gene region. The locations of the kanamycin resistance cassette insertions within vnfY and ORF2 are indicated, together with the denomination (DJ) of the resulting mutant strain. S, SalI; X, XhoI.

View larger version (69K): [in this window] [in a new window]   FIG. 2. Amino acid sequence alignment of VnfY, VnfX, NifX, NafY, and NifY proteins from A. vinelandii. The amino acid sequences are indicated by the single-letter code. Amino acid residues identical or similar in three or more of the aligned proteins are shaded in gray.

View larger version (112K): [in this window] [in a new window]   FIG. 3. Phosphorimage analysis of a native anoxic gel of extracts from A. vinelandii mutant strains. Mutant strains were grown and vnf derepressed in the presence of 49VCl5, as described previously (16). A total of 900 µg of protein was loaded in each lane. Lane 1, CA12 (nifHDK); lane 2, CA11.1 (nifHDKvnfDGK::spc); lane 3, DJ1293 (nifDKvnfY::Kan).

The dinitrogenase and dinitrogenase reductase activities in crude extracts of A. vinelandii strain DJ1293 were also determined and compared to those in extracts of strains CA12 and DJ54 (Table 2). Dinitrogenase and dinitrogenase reductase activities in cell extracts were obtained after titration with an excess of the complementary component as described previously (17). The specific activity of each protein is defined as nanomoles of ethylene formed per minute per milligram of protein in the extract. Extracts of strain DJ1293 were only able to reduce 1.3 nmol of acetylene/min/mg of protein when saturating amounts of dinitrogenase reductase were included in the assay. This value compares to 10 to 15 nmol of acetylene/min/mg of protein reduced by extracts of strains DJ54 and CA12, both wild-type strains for the vnf nitrogenase system. This result is in accordance with the levels of ⁴⁹V radiolabel observed to be associated with vnf dinitrogenase in strains DJ1293 and CA12. Conversely, dinitrogenase reductase activity levels were in the same range in extracts of the DJ1293, DJ54, and CA12 strains, indicating that the mutation in vnfY does not affect vnf dinitrogenase reductase.

It is not surprising that VnfY might have more than one role in the biosynthesis of FeV-co. As noted above, some members of this family of proteins show functional versatility and seem to be involved in more than the binding of FeMo-co or FeV-co precursors only. For example, NifX and NifY have been proposed to have a role in balancing nif gene expression in Klebsiella pneumoniae (6, 20), and NafY acts like a chaperone that stabilizes the apo form of the nif dinitrogenase in A. vinelandii (7, 14). However, VnfY neither seems to regulate the expression of the vnf gene (since a vnfY mutant contains normal levels of VnfDGK protein) nor seems to act as a chaperone because it is not found associated with purified apo-VnfDGK (4).

Unlike the situation observed for the loss of NifY, NafY, NifX, or VnfX function, loss of VnfY function has a clear effect on the maturation of V-containing dinitrogenase which is reflected in a lower level of incorporation of FeV-co into the V-containing dinitrogenase and, consequently, in lower dinitrogenase activity. The vnfY mutant strain is clearly and consistently defective in V-dependent diazotrophic growth when tested in solid medium (data not shown). These effects are not due to a polar effect of the insertion mutation within vnfY on the ORF2, because insertional inactivation of ORF2 does not affect V-dependent diazotrophic growth (data not shown). These observations should provide a physiological and biochemical basis for determining the specific role of VnfY in V-containing dinitrogenase maturation, which should in turn provide insight into the possible roles of this family of proteins in the assembly and insertion of complex metalloclusters.

	ACKNOWLEDGMENTS

 
We thank Carolyn S. Brown for helping grow A. vinelandii strains.

This work was supported by grant GM35332 from NIGMS, National Institutes of Health (to P.W.L.), and grant MCB-9630127, National Science Foundation (to D.R.D).

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Plant and Microbial Biology, University of California—Berkeley, 211 Koshland Hall, Berkeley, CA 94720. Phone: (510) 643-3940. Fax: (510) 642-4995. E-mail: pludden{at}nature.berkeley.edu.

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