Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors.
First-generation interaction maps of Src homology 2 (SH2) domains with receptor tyrosine kinase (RTK) phosphosites have previously been generated using protein microarray (PM) technologies. Here, we developed a large-scale fluorescence polarization (FP) methodology that was able to characterize inte...
| Main Authors: | , , , , , |
|---|---|
| Format: | Article |
| Language: | English |
| Published: |
Public Library of Science (PLoS)
2012-01-01
|
| Series: | PLoS ONE |
| Online Access: | http://europepmc.org/articles/PMC3433420?pdf=render |
| id |
doaj-1941f36962b34cb2a4bf527eecd278e7 |
|---|---|
| record_format |
Article |
| spelling |
doaj-1941f36962b34cb2a4bf527eecd278e72020-11-25T00:23:26ZengPublic Library of Science (PLoS)PLoS ONE1932-62032012-01-0179e4447110.1371/journal.pone.0044471Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors.Ronald J HauseKin K LeungJohn L BarkingeMark F CiaccioChih-Pin ChuuRichard B JonesFirst-generation interaction maps of Src homology 2 (SH2) domains with receptor tyrosine kinase (RTK) phosphosites have previously been generated using protein microarray (PM) technologies. Here, we developed a large-scale fluorescence polarization (FP) methodology that was able to characterize interactions between SH2 domains and ErbB receptor phosphosites with higher fidelity and sensitivity than was previously achieved with PMs. We used the FP assay to query the interaction of synthetic phosphopeptides corresponding to 89 ErbB receptor intracellular tyrosine sites against 93 human SH2 domains and 2 phosphotyrosine binding (PTB) domains. From 358,944 polarization measurements, the affinities for 1,405 unique biological interactions were determined, 83% of which are novel. In contrast to data from previous reports, our analyses suggested that ErbB2 was not more promiscuous than the other ErbB receptors. Our results showed that each receptor displays unique preferences in the affinity and location of recruited SH2 domains that may contribute to differences in downstream signaling potential. ErbB1 was enriched versus the other receptors for recruitment of domains from RAS GEFs whereas ErbB2 was enriched for recruitment of domains from tyrosine and phosphatidyl inositol phosphatases. ErbB3, the kinase inactive ErbB receptor family member, was predictably enriched for recruitment of domains from phosphatidyl inositol kinases and surprisingly, was enriched for recruitment of domains from tyrosine kinases, cytoskeletal regulatory proteins, and RHO GEFs but depleted for recruitment of domains from phosphatidyl inositol phosphatases. Many novel interactions were also observed with phosphopeptides corresponding to ErbB receptor tyrosines not previously reported to be phosphorylated by mass spectrometry, suggesting the existence of many biologically relevant RTK sites that may be phosphorylated but below the detection threshold of standard mass spectrometry procedures. This dataset represents a rich source of testable hypotheses regarding the biological mechanisms of ErbB receptors.http://europepmc.org/articles/PMC3433420?pdf=render |
| collection |
DOAJ |
| language |
English |
| format |
Article |
| sources |
DOAJ |
| author |
Ronald J Hause Kin K Leung John L Barkinge Mark F Ciaccio Chih-Pin Chuu Richard B Jones |
| spellingShingle |
Ronald J Hause Kin K Leung John L Barkinge Mark F Ciaccio Chih-Pin Chuu Richard B Jones Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. PLoS ONE |
| author_facet |
Ronald J Hause Kin K Leung John L Barkinge Mark F Ciaccio Chih-Pin Chuu Richard B Jones |
| author_sort |
Ronald J Hause |
| title |
Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. |
| title_short |
Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. |
| title_full |
Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. |
| title_fullStr |
Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. |
| title_full_unstemmed |
Comprehensive binary interaction mapping of SH2 domains via fluorescence polarization reveals novel functional diversification of ErbB receptors. |
| title_sort |
comprehensive binary interaction mapping of sh2 domains via fluorescence polarization reveals novel functional diversification of erbb receptors. |
| publisher |
Public Library of Science (PLoS) |
| series |
PLoS ONE |
| issn |
1932-6203 |
| publishDate |
2012-01-01 |
| description |
First-generation interaction maps of Src homology 2 (SH2) domains with receptor tyrosine kinase (RTK) phosphosites have previously been generated using protein microarray (PM) technologies. Here, we developed a large-scale fluorescence polarization (FP) methodology that was able to characterize interactions between SH2 domains and ErbB receptor phosphosites with higher fidelity and sensitivity than was previously achieved with PMs. We used the FP assay to query the interaction of synthetic phosphopeptides corresponding to 89 ErbB receptor intracellular tyrosine sites against 93 human SH2 domains and 2 phosphotyrosine binding (PTB) domains. From 358,944 polarization measurements, the affinities for 1,405 unique biological interactions were determined, 83% of which are novel. In contrast to data from previous reports, our analyses suggested that ErbB2 was not more promiscuous than the other ErbB receptors. Our results showed that each receptor displays unique preferences in the affinity and location of recruited SH2 domains that may contribute to differences in downstream signaling potential. ErbB1 was enriched versus the other receptors for recruitment of domains from RAS GEFs whereas ErbB2 was enriched for recruitment of domains from tyrosine and phosphatidyl inositol phosphatases. ErbB3, the kinase inactive ErbB receptor family member, was predictably enriched for recruitment of domains from phosphatidyl inositol kinases and surprisingly, was enriched for recruitment of domains from tyrosine kinases, cytoskeletal regulatory proteins, and RHO GEFs but depleted for recruitment of domains from phosphatidyl inositol phosphatases. Many novel interactions were also observed with phosphopeptides corresponding to ErbB receptor tyrosines not previously reported to be phosphorylated by mass spectrometry, suggesting the existence of many biologically relevant RTK sites that may be phosphorylated but below the detection threshold of standard mass spectrometry procedures. This dataset represents a rich source of testable hypotheses regarding the biological mechanisms of ErbB receptors. |
| url |
http://europepmc.org/articles/PMC3433420?pdf=render |
| work_keys_str_mv |
AT ronaldjhause comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors AT kinkleung comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors AT johnlbarkinge comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors AT markfciaccio comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors AT chihpinchuu comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors AT richardbjones comprehensivebinaryinteractionmappingofsh2domainsviafluorescencepolarizationrevealsnovelfunctionaldiversificationoferbbreceptors |
| _version_ |
1725357060507303936 |