Iron-regulated small RNA expression as Neisseria gonorrhoeae FA 1090 transitions into stationary phase growth

Lydgia A Jackson; Michael Day; Jennie Allen; Edgar Scott 2nd; David W Dyer

doi:10.1186/s12864-017-3684-8

Iron-regulated small RNA expression as Neisseria gonorrhoeae FA 1090 transitions into stationary phase growth

BMC Genomics. 2017 Apr 21;18(1):317. doi: 10.1186/s12864-017-3684-8.

Authors

Lydgia A Jackson¹, Michael Day², Jennie Allen², Edgar Scott 2nd², David W Dyer²

Affiliations

¹ Department of Microbiology and Immunology, University of Oklahoma Health Sciences, 975 NE 10th Street, Oklahoma City, OK 73104, USA. lydgia-jackson@ouhsc.edu.
² Department of Microbiology and Immunology, University of Oklahoma Health Sciences, 975 NE 10th Street, Oklahoma City, OK 73104, USA.

Abstract

Background: For most pathogens, iron (Fe) homeostasis is crucial for maintenance within the host and the ability to cause disease. The primary transcriptional regulator that controls intracellular Fe levels is the Fur (ferric uptake regulator) protein, which exerts its action on transcription by binding to a promoter-proximal sequence termed the Fur box. Fur-regulated transcriptional responses are often fine-tuned at the post-transcriptional level through the action of small regulatory RNAs (sRNAs). Consequently, identifying sRNAs contributing to the control of Fe homeostasis is important for understanding the Fur-controlled bacterial Fe-response network.

Results: In this study, we sequenced size-selected directional libraries representing sRNA samples from Neisseria gonorrhoeae strain FA 1090, and examined the Fe- and temporal regulation of these sRNAs. RNA-seq data for all time points identified a pool of at least 340 potential sRNAs. Differential analysis demonstrated that expression appeared to be regulated by Fe availability for at least fifteen of these sRNAs. Fourteen sRNAs were induced in high Fe conditions, consisting of both cis and trans sRNAs, some of which are predicted to control expression of a known virulence factor, and one SAM riboswitch. An additional putative cis-acting sRNA was repressed by Fe availability. In the pathogenic Neisseria species, one sRNA that contributes to Fe-regulated post-transcriptional control is the Fur-repressible sRNA NrrF. The expression of five Fe-induced sRNAs appeared to be at least partially controlled by NrrF, while the remainder was expressed independently of NrrF. The expression of the 14 Fe-induced sRNAs also exhibited temporal control, as their expression levels increased dramatically as the bacteria entered stationary phase.

Conclusions: Here we report the temporal expression of Fe-regulated sRNAs in N. gonorrhoeae FA 1090 with several appearing to be controlled by the Fe-repressible sRNA NrrF. Temporal regulation of these sRNAs suggests a regulatory role in controlling functions necessary for survival, and may be important for phenotypes often associated with altered growth rates, such as biofilm formation or intracellular survival. Future functional studies will be needed to understand how these regulatory sRNAs contribute to gonococcal biology and pathogenesis.

Keywords: Fur; Iron; Neisseria gonorrhoeae; NrrF; RNA-seq; Riboswitch; Small RNA; Stationary phase; Transcriptome.

MeSH terms

Bacterial Proteins / genetics
Bacterial Proteins / metabolism
Iron / metabolism
Iron / pharmacology*
Neisseria gonorrhoeae / drug effects
Neisseria gonorrhoeae / genetics*
Neisseria gonorrhoeae / growth & development
RNA, Bacterial / chemistry
RNA, Bacterial / isolation & purification
RNA, Bacterial / metabolism*
Riboswitch / drug effects
Riboswitch / genetics
Sequence Analysis, RNA
Transcriptome / drug effects
Virulence Factors / genetics
Virulence Factors / metabolism

Substances

Bacterial Proteins
RNA, Bacterial
Riboswitch
Virulence Factors
Iron

Grants and funding

P20 GM103447/GM/NIGMS NIH HHS/United States