RNA Processing of Nitrogenase Transcripts in the Cyanobacterium<i>Anabaena variabilis</i>

Ungerer, Justin; Pratte, Brenda S.; Thiel, Teresa

doi:10.1128/jb.00278-10

Cited by 31 publications

(78 citation statements)

References 63 publications

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“…A 6-kb SacI fragment of pRL2948a was arrow. The solid rightward arrows indicate transcription start sites (tss) upstream of nifB1, in nifU1, in nifE1, and upstream of hesA1, while the dashed arrows indicate transcription processing sites upstream of nifH1, in ava3935, and upstream of fdxH, as determined previously (33) and in this study. (B) ␤-Galactosidase activities for strains containing fusions of four different regions upstream of nifE1 to a promoterless lacZ.…”

Section: Methodssupporting

confidence: 55%

“…Apparent transcription start sites have been identified upstream of nifB (25,26,(33)(34)(35), nifH (26,36), hesA (30,35), and fdxH (31). Although the putative nifH transcription start site has been identified several times, we were unable to drive transcription of lacZ using a DNA fragment that included the entire niU1-nifH1 intergenic region of A. variabilis, and we showed that the 5= end of the nifH1 transcript in A. variabilis is a processed transcript rather than a transcription initiation site; thus, there is no promoter upstream of nifH1 (33). In contrast, nifB1 has a promoter that initiates transcription, and there is a promoter within the coding region of nifU1 (33), which has been verified by transcriptome sequencing (RNA-seq) (35).…”

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confidence: 99%

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Regulation of Nitrogenase Gene Expression by Transcript Stability in the Cyanobacterium Anabaena variabilis

Pratte

Thiel

2014

Journal of Bacteriology

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The nitrogenase gene cluster in cyanobacteria has been thought to comprise multiple operons; however, in Anabaena variabilis, the promoter for the first gene in the cluster, nifB1, appeared to be the primary promoter for the entire nif cluster. The structural genes nifHDK1 were the most abundant transcripts; however, their abundance was not controlled by an independent nifH1 promoter, but rather, by RNA processing, which produced a very stable nifH1 transcript and a moderately stable nifD1 transcript. There was also no separate promoter for nifEN1. In addition to the nifB1 promoter, there were weak promoters inside the nifU1 gene and inside the nifE1 gene, and both promoters were heterocyst specific. In an xisA mutant, which effectively separated promoters upstream of an 11-kb excision element in nifD1 from the downstream genes, the internal nifE1 promoter was functional. Transcription of the nif1 genes downstream of the 11-kb element, including the most distant genes, hesAB1 and fdxH1, was reduced in the xisA mutant, indicating that the nifB1 promoter contributed to their expression. However, with the exception of nifK1 and nifE1, which had no expression, the downstream genes showed low to moderate levels of transcription in the xisA mutant. The hesA1 gene also had a promoter, but the fdxH gene had a processing site just upstream of the gene. The processing of transcripts at sites upstream of nifH1 and fdxH1 correlated with increased stability of these transcripts, resulting in greater amounts than transcripts that were not close to processing sites.

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Section: Methodssupporting

confidence: 55%

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confidence: 99%

Regulation of Nitrogenase Gene Expression by Transcript Stability in the Cyanobacterium Anabaena variabilis

Pratte

Thiel

2014

Journal of Bacteriology

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“…Demonstrating direct regulation of nifH expression by SigE will require in vitro transcription assays using purified components. However, these experiments are especially challenging because the cis-acting sequences that constitute the nifH promoter have not been identified in Anabaena PCC 7120, and recent data with Anabaena variabilis suggest that multiple distant promoters and RNA-processing events may be involved in expression of the nifHDK operon (50).…”

Section: Discussionmentioning

confidence: 99%

“…The regulation of the Anabaena PCC 7120 nifHDK operon has been studied for over 25 years (14,18,20,43,44,50,53); however, little is known about the transcription components that regulate this operon. Our results suggest that sigE is in -FIG.…”

Section: Discussionmentioning

confidence: 99%

The sigE Gene Is Required for Normal Expression of Heterocyst-Specific Genes in Anabaena sp. Strain PCC 7120

et al. 2011

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The filamentous cyanobacterium Anabaena (Nostoc) sp. strain PCC 7120 produces specialized cells for nitrogen fixation called heterocysts. Previous work showed that the group 2 sigma factor sigE (alr4249; previously called sigF) is upregulated in differentiating heterocysts 16 h after nitrogen step-down. We now show that the sigE gene is required for normal heterocyst development and normal expression levels of several heterocyst-specific genes. Mobility shift assays showed that the transcription factor NtcA binds to sites in the upstream region of sigE and that this binding is enhanced by 2-oxoglutarate (2-OG). Deletions of the region containing the NtcA binding sites in P sigE -gfp reporter plasmids showed that the sites contribute to normal developmental regulation but are not essential for upregulation in heterocysts. Northern RNA blot analysis of nifH mRNA revealed delayed and reduced transcript levels during heterocyst differentiation in a sigE mutant background. Quantitative reverse transcription-PCR (qRT-PCR) analyses of the sigE mutant showed lower levels of transcripts for nifH, fdxH, and hglE2 but normal levels for hupL. We developed a P nifHD -gfp reporter construct that showed strong heterocyst-specific expression. Time-lapse microscopy of the P nifHD -gfp reporter in a sigE mutant background showed delayed development and undetectable green fluorescent protein (GFP) fluorescence. Overexpression of sigE caused accelerated heterocyst development, an increased heterocyst frequency, and premature expression of GFP fluorescence from the P nifHD -gfp reporter.

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“…Ungerer et al (36) reported that the high expression of nifH1 is supported by two promoters: a strong one is located upstream of nifB1, and the other weak one is located in the coding region of nifU1 in A. variabilis. In addition, they pointed out that a secondary structure of 5′ UTR just upstream of nifH1 might contribute to stabilize the processed nifH1 transcript.…”

Section: Discussionmentioning

confidence: 99%

Transcriptional regulators ChlR and CnfR are essential for diazotrophic growth in nonheterocystous cyanobacteria

Tsujimoto¹,

Kamiya

Fujita³

2014

Proc. Natl. Acad. Sci. U.S.A.

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Significance Nitrogen fixation is a process of conversion of atmospheric nitrogen to ammonia catalyzed by nitrogenase, which is quickly inactivated by oxygen. Cyanobacteria are a group of prokaryotes that perform oxygenic photosynthesis, and many cyanobacterial species have the ability to fix nitrogen. How nitrogen fixation is coordinated with oxygenic photosynthesis remains largely unknown. Here we report two transcriptional regulators, ChlR (chlorophyll regulator) and CnfR (cyanobacterial nitrogen fixation regulator), that activate the transcription of genes responsible for anaerobic chlorophyll biosynthesis and the nitrogen fixation genes, respectively, in response to low-oxygen conditions in Leptolyngbya boryana , a diazotrophic cyanobacterium lacking heterocysts.

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RNA Processing of Nitrogenase Transcripts in the CyanobacteriumAnabaena variabilis

Cited by 31 publications

References 63 publications

Regulation of Nitrogenase Gene Expression by Transcript Stability in the Cyanobacterium Anabaena variabilis

Regulation of Nitrogenase Gene Expression by Transcript Stability in the Cyanobacterium Anabaena variabilis

The sigE Gene Is Required for Normal Expression of Heterocyst-Specific Genes in Anabaena sp. Strain PCC 7120

Transcriptional regulators ChlR and CnfR are essential for diazotrophic growth in nonheterocystous cyanobacteria

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