Name: identification of myod interactome using tandem affinity purification coupled to mass spectrometry
Uploaded: 2016-05-17T13:00:00
Description: Watch this Scientific Journal Video about Identification of MyoD Interactome Using Tandem Affinity Purification Coupled to Mass Spectrometry at JoVE.com

Work in the Ait-Si-Ali lab was supported by the Association Fran&#231;aise contre les Myopathies T&#233;l&#233;thon (AFM-T&#233;l&#233;thon); Institut National du Cancer (INCa); Agence Nationale de la Recherche (ANR), Fondation Association pour la Recherche sur le Cancer (Fondation ARC); Groupement des Entreprises Fran&#231;aises pour la Lutte contre le Cancer (GEFLUC); CNRS; Universit&#233; Paris Diderot and the ''Who Am I?'' Laboratory of Excellence #ANR-11- LABX-0071 funded by the French Government through its ''Investments for the Future'' program operated by the ANR under grant #ANR-11-IDEX-0005-01. EB was supported by an INCa grant.

1. Preparation of HeLa-S3 Nuclear Salt-extractable and Chromatin-bound Fractions
<ol>
	<li>Collection of the Cells
	<ol>
		<li>Grow HeLa-S3 Flag-HA-MyoD and HeLa-S3 Flag-HA (control cell line) in Dulbecco&#39;s Modified Eagle Medium (DMEM) supplemented with 10% fetal calf serum, 100 U/ml penicillin and 100 &#181;g/ml streptomycin (growth medium) at 37 &#176;C and 5% CO2 in a humid incubator. 
		Note: HeLa-S3 cells stably expressing Flag-HA-MyoD and HeLa-S3 cells transduced with the empty vector (HeLa-S3...

<ol>
	<li>Ait-Si-Ali, S., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+Suv39h-dependent+mechanism+for+silencing+S-phase+genes+in+differentiating+but+not+in+cycling+cells.">A Suv39h-dependent mechanism for silencing S-phase genes in differentiating but not in cycling cells.</a> Embo J. 23 (3), 605-615 (2004).</li><li>Buckingham, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Skeletal+muscle+development+and+the+role+of+the+myogenic+regulatory+factors.">Skeletal muscle development and the role of the myogenic regulatory factors.</a> Biochem Soc Trans. 24 (2), 506-509 (1996).</li><li>Arnold, H. H., Winter, B. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Muscle+differentiation:+more+complexity+to+the+network+of+myogenic+regulators.">Muscle differentiation: more complexity to the network of myogenic regulators.</a> Curr Opin Genet Dev. 8 (5), 539-544 (1998).</li><li>Buckingham, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Skeletal+muscle+formation+in+vertebrates.">Skeletal muscle formation in vertebrates.</a> Curr Opin Genet Dev. 11 (4), 440-448 (2001).</li><li>Yun, K., Wold, B. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Skeletal+muscle+determination+and+differentiation:+story+of+a+core+regulatory+network+and+its+context.">Skeletal muscle determination and differentiation: story of a core regulatory network and its context.</a> Curr Opin Cell Biol. 8 (6), 877-889 (1996).</li><li>Molkentin, J. D., Olson, E. N. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Defining+the+regulatory+networks+for+muscle+development.">Defining the regulatory networks for muscle development.</a> Curr Opin Genet Dev. 6 (4), 445-453 (1996).</li><li>Arnold, H. H., Braun, T. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Targeted+inactivation+of+myogenic+factor+genes+reveals+their+role+during+mouse+myogenesis:+a+review.">Targeted inactivation of myogenic factor genes reveals their role during mouse myogenesis: a review.</a> Int J Dev Biol. 40 (1), 345-353 (1996).</li><li>Puri, P. L., Sartorelli, V. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Regulation+of+muscle+regulatory+factors+by+DNA-binding,+interacting+proteins,+and+post-transcriptional+modifications.">Regulation of muscle regulatory factors by DNA-binding, interacting proteins, and post-transcriptional modifications.</a> J Cell Physiol. 185 (2), 155-173 (2000).</li><li>Tapscott, S. J. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+circuitry+of+a+master+switch:+Myod+and+the+regulation+of+skeletal+muscle+gene+transcription.">The circuitry of a master switch: Myod and the regulation of skeletal muscle gene transcription.</a> Development. 132 (12), 2685-2695 (2005).</li><li>Lassar, A. B., Paterson, B. M., Weintraub, H. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Transfection+of+a+DNA+locus+that+mediates+the+conversion+of+10T1/2+fibroblasts+to+myoblasts.">Transfection of a DNA locus that mediates the conversion of 10T1/2 fibroblasts to myoblasts.</a> Cell. 47 (5), 649-656 (1986).</li><li>Davis, R. L., Weintraub, H., Lassar, A. B. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Expression+of+a+single+transfected+cDNA+converts+fibroblasts+to+myoblasts.">Expression of a single transfected cDNA converts fibroblasts to myoblasts.</a> Cell. 51, 987-1000 (1987).</li><li>Tapscott, S. J., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=MyoD1:+a+nuclear+phosphoprotein+requiring+a+myc+homology+region+to+convert+fibroblasts+to+myoblasts.">MyoD1: a nuclear phosphoprotein requiring a myc homology region to convert fibroblasts to myoblasts.</a> Science. 242, 405-411 (1988).</li><li>Weintraub, H., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Activation+of+muscle-specific+genes+in+pigment,+nerve,+fat,+liver,+and+fibroblast+cell+lines+by+forced+expression+of+MyoD.">Activation of muscle-specific genes in pigment, nerve, fat, liver, and fibroblast cell lines by forced expression of MyoD.</a> Proc Natl Acad Sci U S A. 86 (14), 5434-5438 (1989).</li><li>Mal, A., Harter, M. L. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=MyoD+is+functionally+linked+to+the+silencing+of+a+muscle-specific+regulatory+gene+prior+to+skeletal+myogenesis.">MyoD is functionally linked to the silencing of a muscle-specific regulatory gene prior to skeletal myogenesis.</a> Proc Natl Acad Sci U S A. 100 (4), 1735-1739 (2003).</li><li>Ohkawa, Y., Marfella, C. G., Imbalzano, A. N. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Skeletal+muscle+specification+by+myogenin+and+Mef2D+via+the+SWI/SNF+ATPase+Brg1.">Skeletal muscle specification by myogenin and Mef2D via the SWI/SNF ATPase Brg1.</a> Embo J. 25 (3), 490-501 (2006).</li><li>Ling, B. M., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Lysine+methyltransferase+G9a+methylates+the+transcription+factor+MyoD+and+regulates+skeletal+muscle+differentiation.">Lysine methyltransferase G9a methylates the transcription factor MyoD and regulates skeletal muscle differentiation.</a> Proc Natl Acad Sci U S A. 109 (3), 841-846 (2012).</li><li>Zhang, C. L., McKinsey, T. A., Olson, E. N. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Association+of+class+II+histone+deacetylases+with+heterochromatin+protein+1:+potential+role+for+histone+methylation+in+control+of+muscle+differentiation.">Association of class II histone deacetylases with heterochromatin protein 1: potential role for histone methylation in control of muscle differentiation.</a> Mol Cell Biol. 22 (20), 7302-7312 (2002).</li><li>Forcales, S. V., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Signal-dependent+incorporation+of+MyoD-BAF60c+into+Brg1-based+SWI/SNF+chromatin-remodelling+complex.">Signal-dependent incorporation of MyoD-BAF60c into Brg1-based SWI/SNF chromatin-remodelling complex.</a> The EMBO journal. 31 (2), 301-316 (2011).</li><li>Nakatani, Y., Ogryzko, V. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Immunoaffinity+purification+of+mammalian+protein+complexes.">Immunoaffinity purification of mammalian protein complexes.</a> Methods Enzymol. 370, 430-444 (2003).</li><li>Ouararhni, K., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+histone+variant+mH2A1.1+interferes+with+transcription+by+down-regulating+PARP-1+enzymatic+activity.">The histone variant mH2A1.1 interferes with transcription by down-regulating PARP-1 enzymatic activity.</a> Genes Dev. 20 (23), 3324-3336 (2006).</li><li>Fritsch, L., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+subset+of+the+histone+H3+lysine+9+methyltransferases+Suv39h1,+G9a,+GLP,+and+SETDB1+participate+in+a+multimeric+complex.">A subset of the histone H3 lysine 9 methyltransferases Suv39h1, G9a, GLP, and SETDB1 participate in a multimeric complex.</a> Mol Cell. 37 (1), 46-56 (2010).</li><li>Robin, P., Fritsch, L., Philipot, O., Svinarchuk, F., Ait-Si-Ali, S. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Post-translational+modifications+of+histones+H3+and+H4+associated+with+the+histone+methyltransferases+Suv39h1+and+G9a.">Post-translational modifications of histones H3 and H4 associated with the histone methyltransferases Suv39h1 and G9a.</a> Genome Biol. 8 (12), R270 (2007).</li><li>Huang da, W., Sherman, B. T., Lempicki, R. A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Systematic+and+integrative+analysis+of+large+gene+lists+using+DAVID+bioinformatics+resources.">Systematic and integrative analysis of large gene lists using DAVID bioinformatics resources.</a> Nat Protoc. 4 (1), 44-57 (2009).</li><li>Huang da, W., Sherman, B. T., Lempicki, R. A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Bioinformatics+enrichment+tools:+paths+toward+the+comprehensive+functional+analysis+of+large+gene+lists.">Bioinformatics enrichment tools: paths toward the comprehensive functional analysis of large gene lists.</a> Nucleic Acids Res. 37 (1), 1-13 (2009).</li><li>Ohta, S., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+protein+composition+of+mitotic+chromosomes+determined+using+multiclassifier+combinatorial+proteomics.">The protein composition of mitotic chromosomes determined using multiclassifier combinatorial proteomics.</a> Cell. 142 (5), 810-821 (2010).</li><li>Yahi, H., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Differential+cooperation+between+heterochromatin+protein+HP1+isoforms+and+MyoD+in+myoblasts.">Differential cooperation between heterochromatin protein HP1 isoforms and MyoD in myoblasts.</a> J Biol Chem. 283 (35), 23692-23700 (2008).</li><li>Philipot, O., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+core+binding+factor+CBF+negatively+regulates+skeletal+muscle+terminal+differentiation.">The core binding factor CBF negatively regulates skeletal muscle terminal differentiation.</a> PloS one. 5 (2), (2010).</li><li>Joliot, V., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+SWI/SNF+subunit/tumor+suppressor+BAF47/INI1+is+essential+in+cell+cycle+arrest+upon+skeletal+muscle+terminal+differentiation.">The SWI/SNF subunit/tumor suppressor BAF47/INI1 is essential in cell cycle arrest upon skeletal muscle terminal differentiation.</a> PloS one. 9 (10), e108858 (2014).</li><li>Tanese, N. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Small-scale+density+gradient+sedimentation+to+separate+and+analyze+multiprotein+complexes.">Small-scale density gradient sedimentation to separate and analyze multiprotein complexes.</a> Methods. 12 (3), 224-234 (1997).</li><li>Singh, K., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+KAP1+phosphorylation+switch+controls+MyoD+function+during+skeletal+muscle+differentiation.">A KAP1 phosphorylation switch controls MyoD function during skeletal muscle differentiation.</a> Genes Dev. 29 (5), 513-525 (2015).</li><li>Cong, L., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Multiplex+genome+engineering+using+CRISPR/Cas+systems.">Multiplex genome engineering using CRISPR/Cas systems.</a> Science. 339 (6121), 819-823 (2013).</li><li>Yahi, H., Philipot, O., Guasconi, V., Fritsch, L., Ait-Si-Ali, S. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Chromatin+modification+and+muscle+differentiation.">Chromatin modification and muscle differentiation.</a> Expert Opin Ther Targets. 10 (6), 923-934 (2006).</li><li>Sun, L., Liu, L., Yang, X. J., Wu, Z. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Akt+binds+prohibitin+2+and+relieves+its+repression+of+MyoD+and+muscle+differentiation.">Akt binds prohibitin 2 and relieves its repression of MyoD and muscle differentiation.</a> J Cell Sci. 117. 117 (Pt 14), 3021-3029 (2004).</li><li>Caretti, G., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=The+RNA+helicases+p68/p72+and+the+noncoding+RNA+SRA+are+coregulators+of+MyoD+and+skeletal+muscle+differentiation.">The RNA helicases p68/p72 and the noncoding RNA SRA are coregulators of MyoD and skeletal muscle differentiation.</a> Dev Cell. 11 (4), 547-560 (2006).</li><li>Knoepfler, P. S., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+conserved+motif+N-terminal+to+the+DNA-binding+domains+of+myogenic+bHLH+transcription+factors+mediates+cooperative+DNA+binding+with+pbx-Meis1/Prep1.">A conserved motif N-terminal to the DNA-binding domains of myogenic bHLH transcription factors mediates cooperative DNA binding with pbx-Meis1/Prep1.</a> Nucleic Acids Res. 27 (18), 3752-3761 (1999).</li><li>Albini, S., Puri, P. L. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=SWI/SNF+complexes,+chromatin+remodeling+and+skeletal+myogenesis:+it's+time+to+exchange!.">SWI/SNF complexes, chromatin remodeling and skeletal myogenesis: it's time to exchange!.</a> Exp Cell Res. 316 (18), 3073-3080 (2010).</li><li>Yahi, H., Fritsch, L., Philipot, O., Guasconi, V., Souidi, M., Robin, P., Polesskaya, A., Losson, R., Harel-Bellan, A., Ait-Si-Ali, S. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Differential+Cooperation+between+Heterochromatin+Protein+HP1+Isoforms+and+MyoD+in+Myoblasts.">Differential Cooperation between Heterochromatin Protein HP1 Isoforms and MyoD in Myoblasts.</a> J Biol Chem. 283 (35), 23692-23700 (2008).</li></ol>

The presented method permits exhaustive identification of partners of a transcription factor, MyoD. It revealed MyoD partners in a heterologous system resistant to MyoD-induced differentiation, namely HeLa-S3 cells. Thus, by definition, identified MyoD partners are ubiquitously expressed. These include general and sequence-specific transcription factors, chromatin-modifying enzymes, RNA processing proteins, kinases (Tables 1 and 2). Since HeLa-S3 cells are resistant to MyoD-induced trans...

Eukaryotic multi-cellular organisms are composed of different organs and tissues. Each functional tissue has a specific gene pattern expression, which is determined at each differentiation step. Cellular differentiation involves activation of specific genes, maintenance of their expression and, generally, silencing of a set of genes such those involved in cell proliferation. Skeletal muscle differentiation, or myogenesis, is thus a multi-step process, that begins with the determination of mesodermal stem cells into myoblasts, and then leads to the terminal differentiation of these myoblasts into first mono-nucleated, and then multi-nucleated, myotubes. Thus, myoblasts are &#34;determined&#34; cells, that are still able to proliferate, but they are committed to the skeletal muscle lineage, and thus can differentiate solely into skeletal muscle cells either during embryonic development or in adult muscle regeneration. The process of skeletal muscle terminal differentiation is orchestrated by a specific genetic program that begins with the permanent exit from the cell cycle of myoblast precursor cells that leads to a definitive silencing of proliferation associated genes, such as E2F target genes1. Indeed, during the process of terminal differentiation, myoblast proliferation arrest is a crucial step that precedes the expression of skeletal muscle specific genes and the fusion of myoblasts into myotubes2. Such a program permits adult muscle stem cells, also called satellite cells, to differentiate during the regeneration process following skeletal muscle injury.
Mammalian myogenesis is critically dependent on a family of myogenic basic helix-loop-helix (bHLH) transcription factors MyoD, Myf5, MRF4 and Myogenin, frequently referred to as the family of skeletal muscle determination factors or MRFs (Muscle Regulatory Factors)3. Each of them plays an essential role in specification and differentiation of skeletal muscle cells and has a specific expression pattern45-7. The activation of Myf5 and MyoD constitutes the determinative step that commits cells to the myogenic lineage, and subsequent expression of Myogenin triggers myogenesis with activation of skeletal muscle specific genes, such as MCK (Muscle Creatine Kinase). Myogenic bHLH transcription factors cooperate with members of the MEF2 family in the activation of muscle genes from previously silent loci8. They also stimulate skeletal muscle gene transcription as heterodimers with ubiquitous bHLH proteins, E12 and E47, known as E proteins, which bind so-called E-boxes in various gene-regulatory regions8. Twist, Id (inhibitor of differentiation) and other factors negatively regulate this process, by competing with MyoD for E proteins binding8.
MyoD is considered as the major player in triggering muscle terminal differentiation9 since it has the capacity to induce a myogenic determination/differentiation (trans-differentiation) program in many fully differentiated non-muscle systems10-13. Indeed, forced expression of MyoD induces the trans-differentiation of different cellular types even those derived from another embryologic origin12. For example, MyoD can convert hepatocytes, fibroblasts, melanocytes, neuroblasts, and adipocytes into muscle-like cells. The trans-differentiative action of MyoD involves an abnormal activation of the myogenic genetic program (notably its target genes) in a non-muscular environment, concomitant to the silencing of the original genetic program (notably, proliferation genes).
In proliferating myoblasts, MyoD is expressed but is unable to activate its target genes even when it binds to their promoters14-16. Therefore, the requirement for MyoD to be continuously expressed in undifferentiated myoblasts remains quite elusive. MyoD could repress its target genes due to recruitment of repressive chromatin-modifying enzymes in proliferating myoblasts prior to loading of activating chromatin remodeling enzymes14,17. For example, in proliferating myoblasts, MyoD is associated with transcriptional co-repressor KAP-1, histone deacetylases (HDACs) and repressive lysine methyltransferases (KMTs), including histone H3 lysine 9 or H3K9 and H3K27 KMTs, and actively suppress its target genes expression by establishing a locally repressive chromatin structure14,17. Importantly, a recent report indicated that MyoD is itself directly methylated by the H3K9 KMT G9a resulting in inhibition of its transactivating activity16.
The epigenetic mechanisms involved in this trans-differentiation of non-muscle cells by MyoD are largely unknown. Notably, some cell lines are resistant to MyoD-induced trans-differentiation. Thus, in HeLa cells, MyoD is either inactive or even might function as repressor rather than activator of transcription due to lack of expression of the BAF60C subunit of the chromatin remodeling complex SWI/SNF18. This model can thus be of choice to better characterize the mechanisms of MyoD-induced gene repression. It is also suitable to assay the ability of MyoD to induce repressive chromatin environment at its target loci with its associated partners and therefore uncover the MyoD-dependent repressive mechanisms in proliferating myoblasts to fine-tune terminal differentiation.
Here we describe the protocol for the identification of MyoD partners by using Tandem Affinity Purification (TAP-Tag) coupled to mass spectrometry (MS) characterization. The use of HeLa-S3 cells stably expressing Flag-HA-MyoD permitted to get enough material to purify the MyoD complexes from fractionated nuclear extracts. The identification of MyoD partners in the heterologous system was followed by validation in a relevant system.

<table border="0" cellpadding="0" cellspacing="0" width="543">
	<tbody>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Cell lines</td>
			<td style="width:115px;"></td>
			<td style="width:101px;"></td>
			<td style="width:151px;"></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">HeLa-S3</td>
			<td style="width:115px;">ATCC</td>
			<td style="width:101px;">CCL-2.2</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">C2C12</td>
			<td style="width:115px;">ATCC</td>
			<td style="width:101px;">CRL-1772</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Name</td>
			<td style="width:115px;">Company</td>
			<td style="width:101px;">Catalog Number</td>
			<td>Comments</td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Equipment</td>
			<td style="width:115px;"></td>
			<td style="width:101px;"></td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Spinner</td>
			<td style="width:115px;">Corning</td>
			<td style="width:101px;">778531</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">Homogenizer :&#160; Dounce homogenizer&#160;</td>
			<td style="width:115px;">Wheaton</td>
			<td style="width:101px;">432-1273 and 432-1271</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Agitating device for spinners</td>
			<td style="width:115px;">Bellco</td>
			<td style="width:101px;">778531</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Sonicator</td>
			<td style="width:115px;">Diagenode</td>
			<td style="width:101px;">UCD 200</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;">Hemocytometer</td>
			<td style="width:115px;">Marienfeld Superior&#160;</td>
			<td style="width:101px;">640610</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Low-binding tubes</td>
			<td style="width:115px;">Sorenson</td>
			<td style="width:101px;">27210</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Empty spin column</td>
			<td style="width:115px;">Bio-Rad</td>
			<td style="width:101px;">7326204</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Name</td>
			<td style="width:115px;">Company</td>
			<td style="width:101px;">Catalog Number</td>
			<td>Comments</td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Reagents</td>
			<td style="width:115px;"></td>
			<td style="width:101px;"></td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">SDS-polyacrylamide 4-12 %&#160; gel</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">NP0336BOX</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">4X loading buffer&#160;</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">NP0007</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">10X reducing agent</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">NP0004</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Silver staining kit</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">A8592</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Centrifugal filter units, 10K</td>
			<td style="width:115px;">Millipore</td>
			<td style="width:101px;">UFC501024</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">Protein G agarose beads</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">P4691</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Protein A/G&#160; Resin</td>
			<td style="width:115px;">Thermo Scientific</td>
			<td style="width:101px;">53132</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">Flag resin (anti-Flag M2-agarose affinity gel)</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A2220</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">HA resin (monoclonal Anti-HA agarose)</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A2095</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">MNase</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">N3755</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">Flag free peptide (DYKDDDDK)</td>
			<td style="width:115px;">Ansynth Service BV</td>
			<td style="width:101px;">Custom synthesis</td>
			<td>Resuspend up to 4 mg/mL in 50 mM Tris-HCl, pH 7.8</td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">HA free peptide (YPYDVPDYA)</td>
			<td style="width:115px;">Ansynth Service BV</td>
			<td style="width:101px;">Custom synthesis</td>
			<td>Resuspend up to 4 mg/mL in 50 mM Tris-HCl, pH 7.8</td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">Bicinchoninic acid based protein assay kit : BCA kit</td>
			<td style="width:115px;">Thermo Scientific</td>
			<td style="width:101px;">23225</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Protease inhibitors</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">S8830</td>
			<td></td>
		</tr>
		<tr height="51">
			<td height="51" style="height:51px;width:177px;">Luminol-based enhanced chemiluminescence (ECL) HRP substrate</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">34075</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">BSA</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A9647</td>
			<td></td>
		</tr>
		<tr height="68">
			<td height="68" style="height:68px;">Sheared salmon sperm DNA (Deoxyribonucleic acid sodium salt from salmon testes)</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">D1626</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">Spermine tetrahydrochloride</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">S1141</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">Spermidine</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">S0266</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">Glycerol</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">G5516</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">PBS</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">D8537</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">MOPS running buffer</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">NP0001</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">DMEM (high glucose)</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">D0822</td>
			<td>Pre-warm&#160; at 37 &#176;C before use</td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;">Trypsin-EDTA (0.05% phenol red</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">25300-054</td>
			<td></td>
		</tr>
		<tr height="51">
			<td height="51" style="height:51px;">Serum</td>
			<td>GE healthcare life sciences&#160;</td>
			<td style="width:101px;">PAA A15-102</td>
			<td style="width:151px;">Each lot of serum has to be first tested for your cells.</td>
		</tr>
		<tr height="20">
			<td height="20" style="height:20px;">Penicillin and Streptomycin&#160;</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">15140-122</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;">Trypan Blue Solution, 0.4%</td>
			<td style="width:115px;">Life technologies</td>
			<td style="width:101px;">15250-061</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Water (sterile-filtered)</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">W3500</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Name</td>
			<td style="width:115px;">Company</td>
			<td style="width:101px;">Catalog Number</td>
			<td>Comments</td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Antibodies</td>
			<td style="width:115px;"></td>
			<td style="width:101px;"></td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">HA from rat (12CA5)</td>
			<td style="width:115px;">Roche</td>
			<td style="width:101px;">11583816001</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Flag</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A8592</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">MyoD</td>
			<td style="width:115px;">Santa Cruz</td>
			<td>sc-32758</td>
			<td>To use for western blotting</td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">MyoD</td>
			<td style="width:115px;">Santa Cruz</td>
			<td>SC-760</td>
			<td>To use for immunoprecipitation and western blotting</td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">CBFbeta</td>
			<td style="width:115px;">Santa Cruz</td>
			<td style="width:101px;">FL-182&#160;</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">HP1alpha</td>
			<td style="width:115px;">Euromedex</td>
			<td style="width:101px;">2HP2G9</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">HP1beta</td>
			<td style="width:115px;">Euromedex</td>
			<td style="width:101px;">1MOD1A9AS</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">HP1gamma</td>
			<td style="width:115px;">Euromedex</td>
			<td style="width:101px;">2MOD1GC</td>
			<td></td>
		</tr>
		<tr height="34">
			<td height="34" style="height:34px;width:177px;">Suv39h1</td>
			<td style="width:115px;">Cell Signaling Technology</td>
			<td style="width:101px;">8729</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">BAF47</td>
			<td style="width:115px;">BD Biosciences</td>
			<td style="width:101px;">612111</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Myf5</td>
			<td style="width:115px;">Santa Cruz</td>
			<td>SC-302</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Tubulin</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">T9026</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Actin</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A5441</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">IgG Mouse</td>
			<td style="width:115px;">Santa Cruz</td>
			<td style="width:101px;">SC-2025</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">IgG Rabbit</td>
			<td style="width:115px;">Santa Cruz</td>
			<td style="width:101px;">SC-2027</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Goat anti-rat -HRP</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A9037</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Goat anti-rabbit -HRP</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A6154&#160;</td>
			<td></td>
		</tr>
		<tr height="17">
			<td height="17" style="height:17px;width:177px;">Goat anti-mouse -HRP</td>
			<td style="width:115px;">Sigma-Aldrich</td>
			<td style="width:101px;">A4416</td>
			<td></td>
		</tr>
	</tbody>
</table>

identification of myod interactome using tandem affinity purification coupled to mass spectrometry

Skeletal muscle terminal differentiation starts with the commitment of pluripotent mesodermal precursor cells to myoblasts. These cells have still the ability to proliferate or they can differentiate and fuse into multinucleated myotubes, which maturate further to form myofibers. Skeletal muscle terminal differentiation is orchestrated by the coordinated action of various transcription factors, in particular the members of the Muscle Regulatory Factors or MRFs (MyoD, Myogenin, Myf5, and MRF4), also called the myogenic bHLH transcription factors family. These factors cooperate with chromatin-remodeling complexes within elaborate transcriptional regulatory network to achieve skeletal myogenesis. In this, MyoD is considered the master myogenic transcription factor in triggering muscle terminal differentiation. This notion is strengthened by the ability of MyoD to convert non-muscle cells into skeletal muscle cells. Here we describe an approach used to identify MyoD protein partners in an exhaustive manner in order to elucidate the different factors involved in skeletal muscle terminal differentiation. The long-term aim is to understand the epigenetic mechanisms involved in the regulation of skeletal muscle genes, i.e., MyoD targets. MyoD partners are identified by using Tandem Affinity Purification (TAP-Tag) from a heterologous system coupled to mass spectrometry (MS) characterization, followed by validation of the role of relevant partners during skeletal muscle terminal differentiation. Aberrant forms of myogenic factors, or their aberrant regulation, are associated with a number of muscle disorders: congenital myasthenia, myotonic dystrophy, rhabdomyosarcoma and defects in muscle regeneration. As such, myogenic factors provide a pool of potential therapeutic targets in muscle disorders, both with regard to mechanisms that cause disease itself and regenerative mechanisms that can improve disease treatment. Thus, the detailed understanding of the intermolecular interactions and the genetic programs controlled by the myogenic factors is essential for the rational design of efficient therapies.

To understand the regulation of MyoD activity, we undertook the exhaustive characterization of the MyoD complexes using biochemical purification, based on the immunopurification of a double tagged form of MyoD followed by mass spectrometry (MS). The use of HeLa-S3 cell line expressing Flag-HA-tagged MyoD and a control cell line expressing Flag-HA permits to get enough material to purify the MyoD complex by performing double-affinity purification of Flag-HA-MyoD.
<p class="jove_content...

Watch this Scientific Journal Video about Identification of MyoD Interactome Using Tandem Affinity Purification Coupled to Mass Spectrometry at JoVE.com

Identification of MyoD Interactome Using Tandem Affinity Purification Coupled to Mass Spectrometry

MyoD is a myogenic transcription factor with a strong capacity to induce myogenic transdifferentiation of many fully differentiated non-muscle cell lines. The epigenetic mechanisms involved in this transdifferentiation are largely unknown. Here we describe a double-affinity purification method followed by mass spectrometry to exhaustively characterize MyoD partners.

Skeletal muscle terminal differentiation starts with the commitment of pluripotent mesodermal precursor cells to myoblasts. These cells have still the ...

The overall goal of this experiment is to exhaustively characterize MyoD protein partners. This method can answer key questions in the skeletal muscle biology field such as molecular regulation of skeletal muscle tonal deformation by the key muscle transcription factor, MyoD. The main advantage of this technique is that it allows us to unravel MyoD partners that have electively low abundance, one localized in one specific subnuclear compartment.Though this method can provide insight into regulation of the muscle differentiation, it can also be applied to other systems, such as any other tissues, specifically nuclear differentiation. Demonstrating the procedure will be Dr.Lauriane Fritsch, a research assistant from our laboratory. In this protocol, MyoD complexes will be purified from HeLa S3 cells that stably express MyoD with FLAG glutenin tags.HeLa S3 cells transduced with the empty vector will be used as the control. Both cell lines were previously grown, collected and stored at negative 80 degrees Celsius, as described in the protocol text. Quickly, thaw the cell pellets in a water bath at 37 degrees Celsius.All buffers and homogenizers should be prechilled and this entire procedure should be performed in a cold room. Typically, 20 grams of cells are used for each experimental point, but for the purposes of this demonstration, only 10 grams, or about 10 mL of cells will be processed. Resuspend the cells in 10 mL of hypotonic buffer A, by using 5 mL of the buffer at first.Then, adding 2.5 mL, followed by another 2.5 mL. Wash the pipette well with fresh buffer to get the maximum of cells. Transfer 20 mL of the cell suspension into the prechilled homogenizer with a tight fitting pestle.Homogenize the cells with 20 strokes. Transfer the cell suspension into a 50 milliliter tube. For maximal recovery of cells, wash the homogenizer with 3.5 mL of sucrose buffer.Transfer this suspension quickly into the 50 mL tube to preserve the nuclei and to limit leakage. Stain a 30 microliter aliquot of the cell suspension with 30 microliters of 4%Trypan Blue and analyze under the microscope to determine the lysis efficiency. All nuclei should be blue if the lysis is successful.If necessary, repeat the homogenization. Centrifuge for seven minutes at 10, 000 x g and four degrees Celsius to pellet the nuclei. Save the supernatant as a cytoplasmic fraction.Begin the procedure for preparing the nuclear salt extractable fraction by resuspending the nuclei pellet in 4 mL of sucrose buffer. Then, add 4 mL of high salt buffer drop by drop while mixing thoroughly on a vortex to get a final concentration of 300 mM sodium chloride. Incubate for 30 minutes on ice with mixing every five minutes.Next, decrease the sodium chloride concentration to 150 mM by adding 8 mL of sucrose buffer. Centrifuge for 10 minutes at 13, 000 x g and four degrees Celsius. Collect the supernatant which is the salt extractable fraction and leave it on ice.To prepare the chromatin bound fraction, resuspend the pellet meticulously in 3.5 mL of sucrose buffer. Add calcium chloride to a final concentration of 1 mM and mix. The calcium chloride will activate the micrococcal nuclease that will be added later.Preheat the suspension for one minute at 37 degrees Celsius. Add 35 microliters of a 5 units per microliter micrococcal nuclease stock to get a final concentration of 25 10 thousandth unit per microliter. Incubate for exactly 12 minutes at 37 degrees Celsius.Mix every four minutes. After 12 minutes, immediately place the reaction on ice. To stop micrococcal nuclease activity, add 56 microliters of 5 molar EDTA pH 8.0 to a final concentration of 4 mM and vortex.Incubate for five minutes on ice. Sonicate five times for one minute each time at high amplitude allowing a break of one minute between sonications. Alter centrifuge both the salt extractable and the nucleosome enriched fractions for 30 minutes at 85, 000 x g at four degrees Celsius.Collect the supernatants. The salt extractable fraction should be about 13 mL. And the nucleasome enriched fraction should be about 6 mL.MyoD protein complexes will be purified by double affinity purification. Since the procedures for FLAG based and HA based purification are similar, only the FLAG based purification will be demonstrated. After adding TEGN transfer the appropriate volume of FLAG resin into a 50 mL tube.300 microliters of FLAG resin from the commercial 50%stock prewash FLAG resin is needed for each experimental point. Centrifuge for two minutes at 1, 000 x g. Remove the supernatant, add cold TEGN, and centrifuge again.Wash the FLAG resin with cold TEGN a total of five times. After the last wash, resuspend the FLAG resin in an equal volume of TEGN. For each experimental point, mix 300 microliters of washed FLAG resin and the corresponding protein extract.Use a 15 mL tube for the nucleasome enriched fraction and a 50 mL tube for the salt extractable fraction. Incubate the tubes on a rotating wheel overnight at four degrees Celsius. On the following day, centrifuge all tubes for two minutes at 1, 000 x g at four degrees Celsius.Collect the supernatants and keep at four degrees Celsius until the result of the purification efficiency test is obtained. For the salt extractable samples, resuspend the FLAG resin in 4 mL of TEGN and transfer to a 15 mL tube. Repeat this step three times, each time transferring to the same 15 mL to avoid losing beads.Centrifuge for two minutes at 1, 000 x g at four degrees Celsius. After removing the supernatant, add 13 mL of TEGN to the FLAG resin and centrifuge for two minutes at 1, 000 x g at four degrees Celsius. Wash the resin seven times in this manner.After the last wash, resuspend the resin in 1 mL of TEGN and transfer into a 1.5 mL low binding tube. Centrifuge for two minutes and remove the supernatant. Resuspend the resin for each experimental point in 100 microliters of FLAG peptide solution at 4 mg/mL at pH 7.8 Mix well and add 100 microliters of TEGN buffer.Incubate at four degrees Celsius for at least four hours to elute bound proteins. Centrifuge for two minutes and transfer the resin and supernatant to an empty spin column placed in a 2 mL tube. Centrifuge the column for one minute at 6, 000 x g.Collect the leftover supernatant in the 2 mL tube. Purification efficiency is then tested as described in the protocol text, before proceeding with HA based purification. Shown here are representative results of double affinity purified MyoD complexes from nuclear salt extractable or nucleasome enriched fractions of a HeLa S3 cell line stably expressing FLAG HA MyoD.Silver staining identified FLAG HA MyoD indicated by the arrow which is absent from the mock cell line. The double affinity purified MyoD complexes were fractionated on glycerol gradients. Western blotting of the fractions using anti-FLAG antibodies uncovered the MyoD subcomplexes in the two subnuclear compartments.In particular, salt extractable MyoD is distributed in three subcomplexes while the chromatin-bound MyoD belongs mainly to one complex. Mass spectrometry analysis of MyoD interactors isolated from nuclear salt extractable and nucleosome enriched fractions identified a series of known partners and new partners of MyoD. Here the MyoD interactors found in both fractions or, specifically for one of the fractions, are grouped based on their functional annotations.Some of the mass spectrometry revealed interactors were confirmed by Western blot on MyoD complexes. These include the transcription factors CBF, the SWI/SNF subunit BAF47 and HP1 proteins. Since HeLa cells are not muscle cells and do not normally express MyoD, it is necessary to confirm interactions between newly identified interactors and MyoD and myoblasts.Nuclear total extracts from proliferating and differentiating mouse myoblasts were used for immunoprecipitation and Western analysis with the indicated antibodies. Once mastered, this technique can be done in two and a half days if it is performed properly. While attempting this procedure, it is important to remember to refine obtained results in myoblasts.Following this procedure, other methods like knockdown of the particular partner in relevance system like myoblasts, can be performed in order to answer additional questions like functional meaning of the interaction. After it's development, this technique paves the way for researchers in the field of developmental biological epigenetics to explore the regulation network of five transcription factors in most body systems. After watching this video, you should have a good understanding of how to identify the partners of for transcription factor by performing cell fractionation followed by tandem affinity purification coupled with mass spectrometry.

identification-myod-interactome-using-tandem-affinity-purification

Research

JoVE Journal

Biology

MALDI Sample Preparation: the Ultra Thin Layer Method

This video demonstrates the preparation of an ultra-thin matrix/analyte layer for analyzing peptides and proteins by Matrix-Assisted Laser Desorption Ionization Mass Spectrometry (MALDI-MS) 1,2. The ultra-thin layer method involves the production of a substrate layer of matrix crystals (alpha-cyano-4-hydroxycinnamic acid) on the sample plate, which serves as a seeding ground for subsequent crystallization of a matrix/analyte mixture. Advantages of the ultra-thin layer method over other sample deposition approaches (e.g. dried droplet) are that it provides (i) greater tolerance to impurities such as salts and detergents, (ii) better resolution, and (iii) higher spatial uniformity. This method is especially useful for the accurate mass determination of proteins. The protocol was initially developed and optimized for the analysis of membrane proteins and used to successfully analyze ion channels, metabolite transporters, and receptors, containing between 2 and 12 transmembrane domains 2. Since the original publication, it has also shown to be equally useful for the analysis of soluble proteins. Indeed, we have used it for a large number of proteins having a wide range of properties, including those with molecular masses as high as 380 kDa 3. It is currently our method of choice for the molecular mass analysis of all proteins. The described procedure consistently produces high-quality spectra, and it is sensitive, robust, and easy to implement.

This video demonstrates the preparation of an ultra-thin matrix/analyte layer for analyzing peptides and proteins by Matrix-Assisted Laser Desorption Ionization Mass Spectrometry (MALDI-MS).

This video demonstrates the preparation of an ultra-thin matrix/analyte layer for analyzing peptides and proteins by Matrix-Assisted Laser Desorption ...

A Quantitative Assessment of The Yeast Lipidome using Electrospray Ionization Mass Spectrometry

Lipids are one of the major classes of biomolecules and play important roles membrane dynamics, energy storage, and signalling1-4. The budding yeast Saccharomyces cerevisiae, a genetically and biochemically manipulable unicellular eukaryote with annotated genome and very simple lipidome, is a valuable model for studying biological functions of various lipid species in multicellular eukaryotes2,3,5. S. cerevisiae has 10 major classes of lipids with chain lengths mainly of 16 or 18 carbon atoms and either zero or one degree of unsaturation6,7. Existing methods for lipid identification and quantification - such as high performance liquid chromatography, thin-layer chromatography, fluorescence microscopy, and gas chromatography followed by MS - are well established but have low sensitivity, insufficiently separate various molecular forms of lipids, require lipid derivitization prior to analysis, or can be quite time consuming. Here we present a detailed description of our experimental approach to solve these inherent limitations by using survey-scan ESI/MS for the identification and quantification of the entire complement of lipids in yeast cells. The described method does not require chromatographic separation of complex lipid mixtures recovered from yeast cells, thereby greatly accelerating the process of data acquisition. This method enables lipid identification and quantification at the concentrations as low as g/ml and has been successfully applied to assessing lipidomes of whole yeast cells and their purified organelles. Lipids extraction from whole yeast cells for using this method of lipid analysis takes two to three hours. It takes only five to ten minutes to run each sample of extracted and dried lipids on a Q-TOF mass spectrometer equipped with a nano-electrospray source.

We describe a new quantitative lipidomics method for identifying numerous lipid species in yeast using survey-scan electrospray ionization mass spectrometry (ESI/MS). This method exceeds currently available methods for lipid identification and quantification in the ability to resolve various molecular forms of lipids, sensitivity, and speed.

Lipids are one of the major classes of biomolecules and play important roles membrane dynamics, energy storage, and signalling1-4. The budding yeast ...

Analyzing Large Protein Complexes by Structural Mass Spectrometry

Living cells control and regulate their biological processes through the coordinated action of a large number of proteins that assemble themselves into an array of dynamic, multi-protein complexes1. To gain a mechanistic understanding of the various cellular processes, it is crucial to determine the structure of such protein complexes, and reveal how their structural organization dictates their function. Many aspects of multi-protein complexes are, however, difficult to characterize, due to their heterogeneous nature, asymmetric structure, and dynamics. Therefore, new approaches are required for the study of the tertiary levels of protein organization.
One of the emerging structural biology tools for analyzing macromolecular complexes is mass spectrometry (MS)2-5. This method yields information on the complex protein composition, subunit stoichiometry, and structural topology. The power of MS derives from its high sensitivity and, as a consequence, low sample requirement, which enables examination of protein complexes expressed at endogenous levels. Another advantage is the speed of analysis, which allows monitoring of reactions in real time. Moreover, the technique can simultaneously measure the characteristics of separate populations co-existing in a mixture. 
Here, we describe a detailed protocol for the application of structural MS to the analysis of large protein assemblies. The procedure begins with the preparation of gold-coated capillaries for nanoflow electrospray ionization (nESI). It then continues with sample preparation, emphasizing the buffer conditions which should be compatible with nESI on the one hand, and enable to maintain complexes intact on the other. We then explain, step-by-step, how to optimize the experimental conditions for high mass measurements and acquire MS and tandem MS spectra. Finally, we chart the data processing and analyses that follow. Rather than attempting to characterize every aspect of protein assemblies, this protocol introduces basic MS procedures, enabling the performance of MS and MS/MS experiments on non-covalent complexes. Overall, our goal is to provide researchers unacquainted with the field of structural MS, with knowledge of the principal experimental tools.

Mass spectrometry has proven to be a valuable tool for analyzing large protein complexes. This method enables insights into the composition, stoichiometry and overall architecture of multi-subunit assemblies. Here, we describe, step-by-step, how to perform a structural mass spectrometry analysis, and characterize macromolecular structures.

Living cells control and regulate their biological processes through the coordinated action of a large number of proteins that assemble themselves into an ...

Quantification of Proteins Using Peptide Immunoaffinity Enrichment Coupled with Mass Spectrometry

There is a great need for quantitative assays in measuring proteins. Traditional sandwich immunoassays, largely considered the gold standard in quantitation, are associated with a high cost, long lead time, and are fraught with drawbacks (e.g. heterophilic antibodies, autoantibody interference, 'hook-effect').1 An alternative technique is affinity enrichment of peptides coupled with quantitative mass spectrometry, commonly referred to as SISCAPA (Stable Isotope Standards and Capture by Anti-Peptide Antibodies).2 In this technique, affinity enrichment of peptides with stable isotope dilution and detection by selected/multiple reaction monitoring mass spectrometry (SRM/MRM-MS) provides quantitative measurement of peptides as surrogates for their respective proteins. SRM/MRM-MS is well established for accurate quantitation of small molecules 3, 4 and more recently has been adapted to measure the concentrations of proteins in plasma and cell lysates.5-7 To achieve quantitation of proteins, these larger molecules are digested to component peptides using an enzyme such as trypsin. One or more selected peptides whose sequence is unique to the target protein in that species (i.e. "proteotypic" peptides) are then enriched from the sample using anti-peptide antibodies and measured as quantitative stoichiometric surrogates for protein concentration in the sample. Hence, coupled to stable isotope dilution (SID) methods (i.e. a spiked-in stable isotope labeled peptide standard), SRM/MRM can be used to measure concentrations of proteotypic peptides as surrogates for quantification of proteins in complex biological matrices. The assays have several advantages compared to traditional immunoassays. The reagents are relatively less expensive to generate, the specificity for the analyte is excellent, the assays can be highly multiplexed, enrichment can be performed from neat plasma (no depletion required), and the technique is amenable to a wide array of proteins or modifications of interest.8-13 In this video we demonstrate the basic protocol as adapted to a magnetic bead platform.

Stable Isotope Standards and Capture by Anti-Peptide Antibodies (SISCAPA) couples affinity enrichment of peptides with stable isotope dilution mass spectrometry (MRM-MS) to provide quantitative measurement of peptides as surrogates for their respective proteins. Here we describe the protocol using magnetic particles in a partially automated format.

There is a great need for quantitative assays in measuring proteins. Traditional sandwich immunoassays, largely considered the gold standard in ...

Orthogonal Protein Purification Facilitated by a Small Bispecific Affinity Tag

Due to the high costs associated with purification of recombinant proteins the protocols need to be rationalized. For high-throughput efforts there is a demand for general methods that do not require target protein specific optimization1 . To achieve this, purification tags that genetically can be fused to the gene of interest are commonly used2 . The most widely used affinity handle is the hexa-histidine tag, which is suitable for purification under both native and denaturing conditions3 . The metabolic burden for producing the tag is low, but it does not provide as high specificity as competing affinity chromatography based strategies1,2.
Here, a bispecific purification tag with two different binding sites on a 46 amino acid, small protein domain has been developed. The albumin-binding domain is derived from Streptococcal protein G and has a strong inherent affinity to human serum albumin (HSA). Eleven surface-exposed amino acids, not involved in albumin-binding4 , were genetically randomized to produce a combinatorial library. The protein library with the novel randomly arranged binding surface (Figure 1) was expressed on phage particles to facilitate selection of binders by phage display technology. Through several rounds of biopanning against a dimeric Z-domain derived from Staphylococcal protein A5, a small, bispecific molecule with affinity for both HSA and the novel target was identified6 .
The novel protein domain, referred to as ABDz1, was evaluated as a purification tag for a selection of target proteins with different molecular weight, solubility and isoelectric point. Three target proteins were expressed in Escherishia coli with the novel tag fused to their N-termini and thereafter affinity purified. Initial purification on either a column with immobilized HSA or Z-domain resulted in relatively pure products. Two-step affinity purification with the bispecific tag resulted in substantial improvement of protein purity. Chromatographic media with the Z-domain immobilized, for example MabSelect SuRe, are readily available for purification of antibodies and HSA can easily be chemically coupled to media to provide the second matrix.
This method is especially advantageous when there is a high demand on purity of the recovered target protein. The bifunctionality of the tag allows two different chromatographic steps to be used while the metabolic burden on the expression host is limited due to the small size of the tag. It provides a competitive alternative to so called combinatorial tagging where multiple tags are used in combination1,7.

A novel and highly efficient two-step affinity chromatography protocol has been developed and is described in detail. The method is based on a small purification tag with two inherent affinities and is applicable to a wide range of target proteins with different properties.

Due to the high costs associated with purification of recombinant proteins the protocols need to be rationalized. For high-throughput efforts there is a ...

Identification of Protein Interacting Partners Using Tandem Affinity Purification

A critical and often limiting step in understanding the function of host and viral proteins is the identification of interacting cellular or viral protein partners. There are many approaches that allow the identification of interacting partners, including the yeast two hybrid system, as well as pull down assays using recombinant proteins and immunoprecipitation of endogenous proteins followed by mass spectrometry identification1. Recent studies have highlighted the utility of double-affinity tag mediated purification, coupled with two specific elution steps in the identification of interacting proteins. This approach, termed Tandem Affinity Purification (TAP), was initially used in yeast2,3 but more recently has been adapted to use in mammalian cells4-8.
As proof-of-concept we have established a tandem affinity purification (TAP) method using the well-characterized eukaryotic translation initiation factor eIF4E9,10.The cellular translation factor eIF4E is a critical component of the cellular eIF4F complex involved in cap-dependent translation initiation10. The TAP tag used in the current study is composed of two Protein G units and a streptavidin binding peptide separated by a Tobacco Etch Virus (TEV) protease cleavage sequence. The TAP tag used in the current study is composed of two Protein G units and a streptavidin binding peptide separated by a Tobacco Etch Virus (TEV) protease cleavage sequence8. To forgo the need for the generation of clonal cell lines, we developed a rapid system that relies on the expression of the TAP-tagged bait protein from an episomally maintained plasmid based on pMEP4 (Invitrogen). Expression of tagged murine eIF4E from this plasmid was controlled using the cadmium chloride inducible metallothionein promoter.
Lysis of the expressing cells and subsequent affinity purification via binding to rabbit IgG agarose, TEV protease cleavage, binding to streptavidin linked agarose and subsequent biotin elution identified numerous proteins apparently specific to the eIF4E pull-down (when compared to control cell lines expressing the TAP tag alone). The identities of the proteins were obtained by excision of the bands from 1D SDS-PAGE and subsequent tandem mass spectrometry. The identified components included the known eIF4E binding proteins eIF4G and 4EBP-1. In addition, other components of the eIF4F complex, of which eIF4E is a component were identified, namely eIF4A and Poly-A binding protein. The ability to identify not only known direct binding partners as well as secondary interacting proteins, further highlights the utility of this approach in the characterization of proteins of unknown function.

Tandem affinity purification is a robust approach for the identification of protein binding partners. As proof of concept, this methodology was applied to the well-characterized translation initiation factor eIF4E to co-precipitate the host cell factors involved in translation initiation. This method is easily adapted to any cellular or viral protein.

A critical and often limiting step in understanding the function of host and viral proteins is the identification of interacting cellular or viral protein ...

Profiling Thiol Redox Proteome Using Isotope Tagging Mass Spectrometry

Pseudomonas syringae pv. tomato strain DC3000 not only causes bacterial speck disease in Solanum lycopersicum but also on Brassica species, as well as on Arabidopsis thaliana, a genetically tractable host plant1,2. The accumulation of reactive oxygen species (ROS) in cotyledons inoculated with DC3000 indicates a role of ROS in modulating necrotic cell death during bacterial speck disease of tomato3. Hydrogen peroxide, a component of ROS, is produced after inoculation of tomato plants with Pseudomonas3. Hydrogen peroxide can be detected using a histochemical stain 3'-3' diaminobenzidine (DAB)4. DAB staining reacts with hydrogen peroxide to produce a brown stain on the leaf tissue4. ROS has a regulatory role of the cellular redox environment, which can change the redox status of certain proteins5. Cysteine is an important amino acid sensitive to redox changes. Under mild oxidation, reversible oxidation of cysteine sulfhydryl groups serves as redox sensors and signal transducers that regulate a variety of physiological processes6,7. Tandem mass tag (TMT) reagents enable concurrent identification and multiplexed quantitation of proteins in different samples using tandem mass spectrometry8,9. The cysteine-reactive TMT (cysTMT) reagents enable selective labeling and relative quantitation of cysteine-containing peptides from up to six biological samples. Each isobaric cysTMT tag has the same nominal parent mass and is composed of a sulfhydryl-reactive group, a MS-neutral spacer arm and an MS/MS reporter10. After labeling, the samples were subject to protease digestion. The cysteine-labeled peptides were enriched using a resin containing anti-TMT antibody. During MS/MS analysis, a series of reporter ions (i.e., 126-131 Da) emerge in the low mass region, providing information on relative quantitation. The workflow is effective for reducing sample complexity, improving dynamic range and studying cysteine modifications. Here we present redox proteomic analysis of the Pst DC3000 treated tomato (Rio Grande) leaves using cysTMT technology. This high-throughput method has the potential to be applied to studying other redox-regulated physiological processes.

Reactive oxygen species level is elevated when cells encounter stress conditions. Here we show the example of 3'-3' diaminobenzidine staining as well as cysTMT labeling and mass spectrometry to profile the redox proteome in Pseudomonas syringae treated tomato leaves.

Pseudomonas syringae pv. tomato strain DC3000 not only causes bacterial speck disease in Solanum lycopersicum but also on Brassica species, as well as on ...

Identification of Protein Complexes in Escherichia coli using Sequential Peptide Affinity Purification in Combination with Tandem Mass Spectrometry

Since most cellular processes are mediated by macromolecular assemblies, the systematic identification of protein-protein interactions (PPI) and the identification of the subunit composition of multi-protein complexes can provide insight into gene function and enhance understanding of biological systems1, 2. Physical interactions can be mapped with high confidence vialarge-scale isolation and characterization of endogenous protein complexes under near-physiological conditions based on affinity purification of chromosomally-tagged proteins in combination with mass spectrometry (APMS). This approach has been successfully applied in evolutionarily diverse organisms, including yeast, flies, worms, mammalian cells, and bacteria1-6. In particular, we have generated a carboxy-terminal Sequential Peptide Affinity (SPA) dual tagging system for affinity-purifying native protein complexes from cultured gram-negative Escherichia coli, using genetically-tractable host laboratory strains that are well-suited for genome-wide investigations of the fundamental biology and conserved processes of prokaryotes1, 2, 7. Our SPA-tagging system is analogous to the tandem affinity purification method developed originally for yeast8, 9, and consists of a calmodulin binding peptide (CBP) followed by the cleavage site for the highly specific tobacco etch virus (TEV) protease and three copies of the FLAG epitope (3X FLAG), allowing for two consecutive rounds of affinity enrichment. After cassette amplification, sequence-specific linear PCR products encoding the SPA-tag and a selectable marker are integrated and expressed in frame as carboxy-terminal fusions in a DY330 background that is induced to transiently express a highly efficient heterologous bacteriophage lambda recombination system10. Subsequent dual-step purification using calmodulin and anti-FLAG affinity beads enables the highly selective and efficient recovery of even low abundance protein complexes from large-scale cultures. Tandem mass spectrometry is then used to identify the stably co-purifying proteins with high sensitivity (low nanogram detection limits).
Here, we describe detailed step-by-step procedures we commonly use for systematic protein tagging, purification and mass spectrometry-based analysis of soluble protein complexes from E. coli, which can be scaled up and potentially tailored to other bacterial species, including certain opportunistic pathogens that are amenable to recombineering. The resulting physical interactions can often reveal interesting unexpected components and connections suggesting novel mechanistic links. Integration of the PPI data with alternate molecular association data such as genetic (gene-gene) interactions and genomic-context (GC) predictions can facilitate elucidation of the global molecular organization of multi-protein complexes within biological pathways. The networks generated for E. coli can be used to gain insight into the functional architecture of orthologous gene products in other microbes for which functional annotations are currently lacking.

Identification of Protein Complexes in Escherichia coli using Sequential Peptide Affinity Purification in Combination with Tandem Mass Spectrometry

Affinity purification of tagged proteins in combination with mass spectrometry (APMS) is a powerful method for the systematic mapping of protein interaction networks and for investigating the mechanistic basis of biological processes. Here, we describe an optimized sequential peptide affinity (SPA) APMS procedure developed for the bacterium Escherichia coli that can be used to isolate and characterize stable multi-protein complexes to near homogeneity even starting from low copy numbers per cell.

Since most cellular processes are mediated by macromolecular assemblies, the systematic identification of protein-protein interactions (PPI) and the ...

A Protocol for the Identification of Protein-protein Interactions Based on 15N Metabolic Labeling, Immunoprecipitation, Quantitative Mass Spectrometry and Affinity Modulation

Protein-protein interactions are fundamental for many biological processes in the cell. Therefore, their characterization plays an important role in current research and a plethora of methods for their investigation is available1. Protein-protein interactions often are highly dynamic and may depend on subcellular localization, post-translational modifications and the local protein environment2. Therefore, they should be investigated in their natural environment, for which co-immunoprecipitation approaches are the method of choice3. Co-precipitated interaction partners are identified either by immunoblotting in a targeted approach, or by mass spectrometry (LC-MS/MS) in an untargeted way. The latter strategy often is adversely affected by a large number of false positive discoveries, mainly derived from the high sensitivity of modern mass spectrometers that confidently detect traces of unspecifically precipitating proteins. A recent approach to overcome this problem is based on the idea that reduced amounts of specific interaction partners will co-precipitate with a given target protein whose cellular concentration is reduced by RNAi, while the amounts of unspecifically precipitating proteins should be unaffected. This approach, termed QUICK for QUantitative Immunoprecipitation Combined with Knockdown4, employs Stable Isotope Labeling of Amino acids in Cell culture (SILAC)5 and MS to quantify the amounts of proteins immunoprecipitated from wild-type and knock-down strains. Proteins found in a 1:1 ratio can be considered as contaminants, those enriched in precipitates from the wild type as specific interaction partners of the target protein. Although innovative, QUICK bears some limitations: first, SILAC is cost-intensive and limited to organisms that ideally are auxotrophic for arginine and/or lysine. Moreover, when heavy arginine is fed, arginine-to-proline interconversion results in additional mass shifts for each proline in a peptide and slightly dilutes heavy with light arginine, which makes quantification more tedious and less accurate5,6. Second, QUICK requires that antibodies are titrated such that they do not become saturated with target protein in extracts from knock-down mutants.
Here we introduce a modified QUICK protocol which overcomes the abovementioned limitations of QUICK by replacing SILAC for 15N metabolic labeling and by replacing RNAi-mediated knock-down for affinity modulation of protein-protein interactions. We demonstrate the applicability of this protocol using the unicellular green alga Chlamydomonas reinhardtii as model organism and the chloroplast HSP70B chaperone as target protein7 (Figure 1). HSP70s are known to interact with specific co-chaperones and substrates only in the ADP state8. We exploit this property as a means to verify the specific interaction of HSP70B with its nucleotide exchange factor CGE19.

A Protocol for the Identification of Protein-protein Interactions Based on 15N Metabolic Labeling, Immunoprecipitation, Quantitative Mass Spectrometry and Affinity Modulation

We present a variation of the QUICK (QUantitative Immunoprecipitation Combined with Knockdown) approach that was introduced previously to distinguish between true and false protein-protein interactions. Our approach is based on 15N metabolic labeling, the modulation of affinities of protein-protein interactions by the presence/absence of ATP, immunoprecipitation, and quantitative mass spectrometry.

Protein-protein interactions are fundamental for many biological processes in the cell. Therefore, their characterization plays an important role in ...

High-throughput Purification of Affinity-tagged Recombinant Proteins

X-ray crystallography is the method of choice for obtaining a detailed view of the structure of proteins. Such studies need to be complemented by further biochemical analyses to obtain detailed insights into structure/function relationships. Advances in oligonucleotide- and gene synthesis technology make large-scale mutagenesis strategies increasingly feasible, including the substitution of target residues by all 19 other amino acids. Gain- or loss-of-function phenotypes then allow systematic conclusions to be drawn, such as the contribution of particular residues to catalytic activity, protein stability and/or protein-protein interaction specificity.
In order to attribute the different phenotypes to the nature of the mutation - rather than to fluctuating experimental conditions - it is vital to purify and analyse the proteins in a controlled and reproducible manner. High-throughput strategies and the automation of manual protocols on robotic liquid-handling platforms have created opportunities to perform such complex molecular biological procedures with little human intervention and minimal error rates1-5.
Here, we present a general method for the purification of His-tagged recombinant proteins in a high-throughput manner. In a recent study, we applied this method to a detailed structure-function investigation of TFIIB, a component of the basal transcription machinery. TFIIB is indispensable for promoter-directed transcription in vitro and is essential for the recruitment of RNA polymerase into a preinitiation complex6-8. TFIIB contains a flexible linker domain that penetrates the active site cleft of RNA polymerase9-11. This linker domain confers two biochemically quantifiable activities on TFIIB, namely (i) the stimulation of the catalytic activity during the 'abortive' stage of transcript initiation, and (ii) an additional contribution to the specific recruitment of RNA polymerase into the preinitiation complex4,5,12 . We exploited the high-throughput purification method to generate single, double and triple substitution and deletions mutations within the TFIIB linker and to subsequently analyse them in functional assays for their stimulation effect on the catalytic activity of RNA polymerase4. Altogether, we generated, purified and analysed 381 mutants - a task which would have been time-consuming and laborious to perform manually. We produced and assayed the proteins in multiplicates which allowed us to appreciate any experimental variations and gave us a clear idea of the reproducibility of our results.
This method serves as a generic protocol for the purification of His-tagged proteins and has been successfully used to purify other recombinant proteins. It is currently optimised for the purification of 24 proteins but can be adapted to purify up to 96 proteins.

We describe a method for the affinity-tagged purification of recombinant proteins using liquid-handling robotics. This method is generally applicable to the small-scale purification of soluble His-tagged proteins in a high-throughput format.

X-ray crystallography is the method of choice for obtaining a detailed view of the structure of proteins. Such studies need to be complemented by further ...