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Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis

BACKGROUND: sRNAs, which belong to the non-coding RNA family and range from approximately 50 to 400 nucleotides, serve various important gene regulatory roles. Most are believed to be trans-regulating and function by being complementary to their target mRNAs in order to inhibiting translation by rib...

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Autores principales: Wu, Timothy H, Chang, Ian Yi-Feng, Chu, Li-chieh Julie, Huang, Hsuan-Cheng, Ng, Wailap Victor
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2010
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2957679/
https://www.ncbi.nlm.nih.gov/pubmed/21106118
http://dx.doi.org/10.1186/1471-2105-11-S7-S11
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author Wu, Timothy H
Chang, Ian Yi-Feng
Chu, Li-chieh Julie
Huang, Hsuan-Cheng
Ng, Wailap Victor
author_facet Wu, Timothy H
Chang, Ian Yi-Feng
Chu, Li-chieh Julie
Huang, Hsuan-Cheng
Ng, Wailap Victor
author_sort Wu, Timothy H
collection PubMed
description BACKGROUND: sRNAs, which belong to the non-coding RNA family and range from approximately 50 to 400 nucleotides, serve various important gene regulatory roles. Most are believed to be trans-regulating and function by being complementary to their target mRNAs in order to inhibiting translation by ribosome occlusion. Despite this understanding of their functionality, the global properties associated with regulation by sRNAs are not yet understood. Here we use topological analysis of sRNA targets in terms of protein-protein interaction and transcription-regulatory networks in Escherichia coli to shed light on the global correlation between sRNA regulation and cellular control networks. RESULTS: The analysis of sRNA targets in terms of their networks showed that some specific network properties could be identified. In protein-protein interaction network, sRNA targets tend to occupy more central positions (higher closeness centrality, p-val = 0.022) and more cliquish (larger clustering coefficient, p-val = 0.037). The targets of the same sRNA tend to form a network module (shorter characteristic path length, p-val = 0.015; larger density, p-val = 0.019; higher in-degree ratio, p-val = 0.009). Using the transcription-regulatory network, sRNA targets tend to be under multiple regulation (higher indegree, p-val = 0.013) and the targets usually are important to the transfer of regulatory signals (higher betweenness, p-val = 0.012). As was found for the protein-protein interaction network, the targets that are regulated by the same sRNA also tend to be closely knit within the transcription-regulatory network (larger density, p-val = 0.036), and inward interactions between them are greater than the outward interactions (higher in-degree ratio, p-val = 0.023). However, after incorporating information on predicted sRNAs and down-stream targets, the results are not as clear-cut, but the overall network modularity is still evident. CONCLUSIONS: Our results indicate that sRNA targeting tends to show a clustering pattern that is similar to the human microRNA regulation associated with protein-protein interaction network that was observed in a previous study. Namely, the sRNA targets show close interaction and forms a closely knit network module for both the protein-protein interaction and the transcription-regulatory networks. Thus, targets of the same sRNA work in a concerted way toward a specific goal. In addition, in the transcription-regulatory network, sRNA targets act as "multiplexor", accepting regulatory control from multiple sources and acting accordingly. Our results indicate that sRNA targeting shows different properties when compared to the proteins that form cellular networks.
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spelling pubmed-29576792010-10-21 Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis Wu, Timothy H Chang, Ian Yi-Feng Chu, Li-chieh Julie Huang, Hsuan-Cheng Ng, Wailap Victor BMC Bioinformatics Proceedings BACKGROUND: sRNAs, which belong to the non-coding RNA family and range from approximately 50 to 400 nucleotides, serve various important gene regulatory roles. Most are believed to be trans-regulating and function by being complementary to their target mRNAs in order to inhibiting translation by ribosome occlusion. Despite this understanding of their functionality, the global properties associated with regulation by sRNAs are not yet understood. Here we use topological analysis of sRNA targets in terms of protein-protein interaction and transcription-regulatory networks in Escherichia coli to shed light on the global correlation between sRNA regulation and cellular control networks. RESULTS: The analysis of sRNA targets in terms of their networks showed that some specific network properties could be identified. In protein-protein interaction network, sRNA targets tend to occupy more central positions (higher closeness centrality, p-val = 0.022) and more cliquish (larger clustering coefficient, p-val = 0.037). The targets of the same sRNA tend to form a network module (shorter characteristic path length, p-val = 0.015; larger density, p-val = 0.019; higher in-degree ratio, p-val = 0.009). Using the transcription-regulatory network, sRNA targets tend to be under multiple regulation (higher indegree, p-val = 0.013) and the targets usually are important to the transfer of regulatory signals (higher betweenness, p-val = 0.012). As was found for the protein-protein interaction network, the targets that are regulated by the same sRNA also tend to be closely knit within the transcription-regulatory network (larger density, p-val = 0.036), and inward interactions between them are greater than the outward interactions (higher in-degree ratio, p-val = 0.023). However, after incorporating information on predicted sRNAs and down-stream targets, the results are not as clear-cut, but the overall network modularity is still evident. CONCLUSIONS: Our results indicate that sRNA targeting tends to show a clustering pattern that is similar to the human microRNA regulation associated with protein-protein interaction network that was observed in a previous study. Namely, the sRNA targets show close interaction and forms a closely knit network module for both the protein-protein interaction and the transcription-regulatory networks. Thus, targets of the same sRNA work in a concerted way toward a specific goal. In addition, in the transcription-regulatory network, sRNA targets act as "multiplexor", accepting regulatory control from multiple sources and acting accordingly. Our results indicate that sRNA targeting shows different properties when compared to the proteins that form cellular networks. BioMed Central 2010-10-15 /pmc/articles/PMC2957679/ /pubmed/21106118 http://dx.doi.org/10.1186/1471-2105-11-S7-S11 Text en Copyright ©2010 Wu et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Proceedings
Wu, Timothy H
Chang, Ian Yi-Feng
Chu, Li-chieh Julie
Huang, Hsuan-Cheng
Ng, Wailap Victor
Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title_full Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title_fullStr Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title_full_unstemmed Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title_short Modularity of Escherichia coli sRNA regulation revealed by sRNA-target and protein network analysis
title_sort modularity of escherichia coli srna regulation revealed by srna-target and protein network analysis
topic Proceedings
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2957679/
https://www.ncbi.nlm.nih.gov/pubmed/21106118
http://dx.doi.org/10.1186/1471-2105-11-S7-S11
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