User:Anthony Milto/Sandbox 1

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==MyoD==
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<StructureSection load='' size='340' side='right' caption='Crystal Structure of MyoD Homodimer bHLH Domain' scene='71/714943/Myod_bhlh_domain/1'>
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==Function and Classification==
==Function and Classification==
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MyoD, along with Myf5, is responsible for muscle cell differentiation and establishment of the myogenic lineage. It is a member of the basic helix loop helix (bHLH) family and myogenic factors subfamily of proteins[[1]].
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MyoD, along with Myf5, is responsible for muscle cell differentiation and establishment of the myogenic lineage. It is a member of the basic helix loop helix (bHLH) family and myogenic factors subfamily of proteins <ref>Phospho Site Plus. http://www.phosphosite.org/proteinAction.do?id=3637&showAllSites=true (accessed October 6, 2015)</ref>.
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<StructureSection load='1mdy' size='340' side='right' caption='Crystal Structure of MyoD bHLH Domain' scene=''>
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==Structure==
==Structure==
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MyoD has a basic region at its amino-terminal end, which functions in binding the transcription factor to a region of the DNA known as the E-box. At the carboxyl-terminal end is MyoD's HLH domain. The HLH domain functions in protein-protein interactions and forms homodimeric and heterodimeric complexes <ref>PMCID: 463060</ref>.MyoD also contains an acidic activation domain. The activity of this activation domain has been observed to increase drastically upon deletion of residues in other parts of the protein. This suggests that the acidic activation domain is buried within the protein in vivo and can be activated by subtle changes in structure [[3]]. MyoD's ability to activate endogenous genes has been shown to rely on two regions. The first is a region rich in cysteine and histidine residues that is between the acidic activation domain and the bHLH domain. The second is a region near the carboxyl terminus of the protein. These regions are conserved in proteins with shared functionality [[4]].
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MyoD has a basic region at its amino-terminal end, which functions in binding the transcription factor to a region of the DNA known as the E-box. At the carboxyl-terminal end is MyoD's <scene name='71/714943/Hlh/2'>HLH domain</scene>. The HLH domain functions in <scene name='71/714943/Hlh_interaction_segment/5'>protein-protein interactions</scene> and forms homodimeric and heterodimeric complexes through a combination of hydrophobic interactions and hydrogen bonding (hydrophobic residues in gray, hydrogen bonding in purple) <ref>DOI: 10.1186/gb-2004-5-6-226</ref>.MyoD also contains an acidic activation domain. The activity of this activation domain has been observed to increase drastically upon deletion of residues in other parts of the protein. This suggests that the acidic activation domain is buried within the protein in vivo and can be activated by subtle changes in structure <ref>Weintraub, H., Dwarki, V. J., Verma, I., Davis, R., Hollenberg, S., Snider, L., Lassar, A., Tapscott, S. J. Muscle-specific transcriptional activation
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by MyoD. Genes & Dev. '''1991'''. 5. 1377-1386 </ref>.
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==DNA Interaction ==
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MyoD, along with most other bHLH proteins, recognizes the consensus DNA sequence CAN NTG, where N can be any base. This sequence is known as the <scene name='71/714943/E-box/2'>E-box</scene> and is bound by MyoD's <scene name='71/714943/Br_dna_interaction/4'>basic region</scene> (basic residues pictured in blue, acidic in red) in DNA's major groove. MyoD's basic region residues indirectly establish selectivity for specific E-box sequences by influencing the conformation in which the basic region binds DNA. There are <scene name='71/714943/Dna_interacting_aas/1'>four residues</scene> responsible for the DNA interaction that provides MyoD's myogenic effect: Arg111, Ala114, Thr115, and Lys124. The lysine and arginine residues are situated near the backbone of the DNA and interact with the backbone phosphate groups and create a type of phosphate clamp, while the alanine and threonine are in DNA's major groove and interact with the DNA's bases <ref>Kophengnavong, T., Michnowicz, J. E., & Blackwell, T. K. Establishment of Distinct MyoD, E2A, and Twist DNA Binding Specificities by Different Basic Region-DNA Conformations. Molecular and Cellular Biology, '''2000''', 20. 261–272.</ref>.
== Regulation ==
== Regulation ==
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MyoD is subject to regulation at both its bHLH domain and its acidic activation domain. Differences in E-box sequences and in complex formation determine the transcription factor's effect and allow differentiation into a diverse array of muscle cells [[2]]. MyoD is only functional when bound to DNA. It has been proposed that DNA binding, with its accompanying structural changes, is required in vivo to free the acidic activation domain and activate MyoD's myogenic functions [[3]]. MyoD functions as a transcriptional activator only as a heterodimer with E proteins, which are a sub-family of bHLH proteins. This interaction takes place in the bHLH domain of both proteins. In one experiment, forced binding of E12 to MyoD that had been inhibited using E protein fragments substantially restored MyoD's activity [[5]]. The myogenic ability of MyoD is inhibited by the presence of another bHLH protein known as Twist. Twist inhibits MyoD by competitively binding E proteins and preventing MyoD-E protein heterodimers from forming [[6]].
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MyoD is subject to regulation both by complex formation with other proteins and by DNA binding. Differences in E-box sequences, as well as sequences flanking the E-box, and in complex formation determine the transcription factor's effect and allow differentiation into a diverse array of muscle cells <ref>DOI: 10.1186/gb-2004-5-6-226</ref>. MyoD is only functional when bound to DNA. It has been proposed that DNA binding, with its accompanying structural changes, is required in vivo to free the acidic activation domain and activate MyoD's myogenic functions <ref>Weintraub, H., Dwarki, V. J., Verma, I., Davis, R., Hollenberg, S., Snider, L., Lassar, A., Tapscott, S. J. Muscle-specific transcriptional activation by MyoD. Genes & Dev. '''1991'''. 5. 1377-1386 </ref>.
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MyoD functions as a transcriptional activator only as a heterodimer with E proteins, which are a sub-family of bHLH proteins. This interaction takes place in the bHLH domain of both proteins. In one experiment, forced binding of E12 to MyoD that had been inhibited using E protein fragments substantially restored MyoD's activity <ref>doi: 10.1101/gad.1765109</ref>. The myogenic ability of MyoD is inhibited by the presence of another bHLH protein known as Twist. Twist inhibits MyoD by competitively binding E proteins and preventing MyoD-E protein heterodimers from forming <ref>Hamamori, Y., Wu, H. Y., Sartorelli, V., & Kedes, L. The basic domain of myogenic basic helix-loop-helix (bHLH) proteins is the novel target for direct inhibition by another bHLH protein, Twist. Molecular and Cellular Biology. '''1997'''. 17. 6563–6573.</ref>.
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The protein IFRD1 is an activating cofactor of MyoD. This protein and MyoD cooperatively activate muscle-specific enhancers. This same cofactor also represses NF-κB, which has been shown to inhibit MyoD mRNA translation <ref>PMID: 21127072</ref>.
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p300, a histone deacetyltransferase, cooperatively interacts with MyoD in the process of converting fibroblasts to myoblasts. This interaction occurs between MyoD's activation domain and both the amino terminus and carboxy terminus of p300 <ref>PMID: 9001254</ref>.
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MyoD is degraded by ubiquination of its N-terminal Lys residue. Data suggests that this occurs through attachment of ubiquitin at the N-terminal residue, followed by synthesis of a polyubiquitin chain on an internal Lys residue, which sufficiently disrupts MyoD's structure to cause degradation. This process is a major pathway of selective protein degradation in eukaryotic cells <ref>DOI: 10.1093/emboj/17.20.5964</ref>. Ubiquination takes place only when MyoD is hyperphosphorylated at its cyclin-dependent kinase (CDK) sites. These CDK sites are Ser or Thr residues that are preceded by a Pro residue. Ser200 has been demonstrated to be required for MyoD to become hyperphosphorylated <ref>Song, A., Wang, Q., Goebl, M. G., & Harrington, M. A. (1998). Phosphorylation of Nuclear MyoD Is Required for Its Rapid Degradation. Molecular and Cellular Biology. '''1998'''. 18. 4994–4999</ref>.
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==DNA Interaction ==
 
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MyoD, along with most other bHLH proteins, recognizes the concensus DNA sequence CAN NTG, where N can be any base. This sequence is known as the E-box and is bound by MyoD's <scene name='71/714943/Br_dna_interaction/1'>basic region</scene>. MyoD's basic region residues indirectly establish specificity for specific E-box sequences by influencing the conformation in which the basic region binds DNA. There are <scene name='71/714943/Dna_interacting_aas/1'>four residues</scene> responsible for the DNA interaction that provides MyoD's myogenic effect: Arg111, Ala114, Thr115, and Lys124.
 
== Knockout Effects ==
== Knockout Effects ==
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Knockout mutations of the MyoD gene have been shown to produce no distinct skeletal muscle phenotype due to an increase in Myf5 activation. Mutants lacking both MyoD and Myf5 fail to develop skeletal musculature all together (REFERENCE)
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Knockout mutations of the MyoD gene have been shown to produce no distinct skeletal muscle phenotype due to an increase in Myf5 activation. Mutants lacking both MyoD and Myf5 fail to develop skeletal musculature all together <ref>Arnold, H. H.; Braun, T. Targeted inactivation of myogenic factor genes reveals their role during mouse myogenesis: a review. Int. J. Dev. Biol. '''1996'''. 40. 345-353</ref>.
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This is a sample scene created with SAT to <scene name="/12/3456/Sample/1">color</scene> by Group, and another to make <scene name="/12/3456/Sample/2">a transparent representation</scene> of the protein. You can make your own scenes on SAT starting from scratch or loading and editing one of these sample scenes.
 
</StructureSection>
</StructureSection>
== References ==
== References ==
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[http://www.phosphosite.org/proteinAction.do?id=3637&showAllSites=true]
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[http://www.ncbi.nlm.nih.gov/pmc/articles/PMC463060/]
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[http://genesdev.cshlp.org/content/5/8/1377.long]
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[http://genesdev.cshlp.org/content/11/4/436.full.pdf]
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[http://genesdev.cshlp.org/content/23/6/694.full]
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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC232510/
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<references/>
<references/>

Current revision

MyoD

Crystal Structure of MyoD Homodimer bHLH Domain

Drag the structure with the mouse to rotate

References

  1. Phospho Site Plus. http://www.phosphosite.org/proteinAction.do?id=3637&showAllSites=true (accessed October 6, 2015)
  2. Jones S. An overview of the basic helix-loop-helix proteins. Genome Biol. 2004;5(6):226. Epub 2004 May 28. PMID:15186484 doi:http://dx.doi.org/10.1186/gb-2004-5-6-226
  3. Weintraub, H., Dwarki, V. J., Verma, I., Davis, R., Hollenberg, S., Snider, L., Lassar, A., Tapscott, S. J. Muscle-specific transcriptional activation by MyoD. Genes & Dev. 1991. 5. 1377-1386
  4. Kophengnavong, T., Michnowicz, J. E., & Blackwell, T. K. Establishment of Distinct MyoD, E2A, and Twist DNA Binding Specificities by Different Basic Region-DNA Conformations. Molecular and Cellular Biology, 2000, 20. 261–272.
  5. Jones S. An overview of the basic helix-loop-helix proteins. Genome Biol. 2004;5(6):226. Epub 2004 May 28. PMID:15186484 doi:http://dx.doi.org/10.1186/gb-2004-5-6-226
  6. Weintraub, H., Dwarki, V. J., Verma, I., Davis, R., Hollenberg, S., Snider, L., Lassar, A., Tapscott, S. J. Muscle-specific transcriptional activation by MyoD. Genes & Dev. 1991. 5. 1377-1386
  7. Yang Z, MacQuarrie KL, Analau E, Tyler AE, Dilworth FJ, Cao Y, Diede SJ, Tapscott SJ. MyoD and E-protein heterodimers switch rhabdomyosarcoma cells from an arrested myoblast phase to a differentiated state. Genes Dev. 2009 Mar 15;23(6):694-707. doi: 10.1101/gad.1765109. PMID:19299559 doi:http://dx.doi.org/10.1101/gad.1765109
  8. Hamamori, Y., Wu, H. Y., Sartorelli, V., & Kedes, L. The basic domain of myogenic basic helix-loop-helix (bHLH) proteins is the novel target for direct inhibition by another bHLH protein, Twist. Molecular and Cellular Biology. 1997. 17. 6563–6573.
  9. Micheli L, Leonardi L, Conti F, Maresca G, Colazingari S, Mattei E, Lira SA, Farioli-Vecchioli S, Caruso M, Tirone F. PC4/Tis7/IFRD1 stimulates skeletal muscle regeneration and is involved in myoblast differentiation as a regulator of MyoD and NF-kappaB. J Biol Chem. 2011 Feb 18;286(7):5691-707. doi: 10.1074/jbc.M110.162842. Epub 2010, Dec 2. PMID:21127072 doi:http://dx.doi.org/10.1074/jbc.M110.162842
  10. Sartorelli V, Huang J, Hamamori Y, Kedes L. Molecular mechanisms of myogenic coactivation by p300: direct interaction with the activation domain of MyoD and with the MADS box of MEF2C. Mol Cell Biol. 1997 Feb;17(2):1010-26. PMID:9001254
  11. Breitschopf K, Bengal E, Ziv T, Admon A, Ciechanover A. A novel site for ubiquitination: the N-terminal residue, and not internal lysines of MyoD, is essential for conjugation and degradation of the protein. EMBO J. 1998 Oct 15;17(20):5964-73. PMID:9774340 doi:http://dx.doi.org/10.1093/emboj/17.20.5964
  12. Song, A., Wang, Q., Goebl, M. G., & Harrington, M. A. (1998). Phosphorylation of Nuclear MyoD Is Required for Its Rapid Degradation. Molecular and Cellular Biology. 1998. 18. 4994–4999
  13. Arnold, H. H.; Braun, T. Targeted inactivation of myogenic factor genes reveals their role during mouse myogenesis: a review. Int. J. Dev. Biol. 1996. 40. 345-353

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