A RAG1 and RAG2 Tetramer Complex Is Active in Cleavage in V(D)J Recombination

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Molecular and Cellular Biology, July 1999, p. 4664-4671, Vol. 19, No. 7
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

A RAG1 and RAG2 Tetramer Complex Is Active in Cleavage in V(D)J Recombination

Tu Bailin, Xianming Mo, and Moshe J. Sadofsky^*

Program of Gene Regulation, Institute of Molecular Medicine and Genetics, Medical College of Georgia, Augusta, Georgia 30912-2650

Received 29 January 1999/Returned for modification 22 February 1999/Accepted 1 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

During V(D)J recombination two proteins, RAG1 and RAG2, assemble as a protein-DNA complex with the appropriate DNA targetscontaining recombination signal sequences (RSSs). The propertiesof this complex require a fairly elaborate set of protein-proteinand protein-DNA contacts. Here we show that a purified derivativeof RAG1, without DNA, exists predominantly as a homodimer. A RAG2derivative alone has monomer, dimer, and larger forms. The coexpressedRAG1 and RAG2 proteins form a mixed tetramer in solution whichcontains two molecules of each protein. The same tetramer of RAG1and RAG2 plus one DNA molecule is the form active in cleavage.Additionally, we show that both DNA products following cleavagecan still be held together in a stable protein-DNAcomplex.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A site-specific DNA recombination mechanism, termed V(D)J recombination, is used in the developing adaptive immune systemto assemble active rearranged genes for the antigen receptorsfrom arrays of inherited inactive segments (reviewed in references6 and 11). Targets for this recombination reaction are identifiedby recombination signal sequences (RSSs) which specify the recombinationsite in the DNA immediately adjacent to the coding sequences.The RSS is composed of a conserved heptamer (CACAGTG) and nonamer(ACAAAAACC) motif, separated by a spacer of either 12 or 23 bpin length (called 12RSS or 23RSS, respectively). A productiverearrangement in cells always occurs between pairs of DNA segmentsbordered by RSS elements of the two different spacer lengths (the12/23 rule [26]). Within a chromosomal locus, similar segmentsgenerally carry RSSs of the same length. Owing to the 12/23 rule,this organization permits a V segment (for example) to join toa D segment but not a second V segment. Several recent investigationshave shown that binding to individual DNA molecules containingsingle RSS as well as simultaneous binding that obeys the 12/23rule can be mediated by RAG1 and RAG2 (5, 7, 8, 30,31) and is aided by the sequence-nonspecific DNA bending proteinHMG1 (9, 21, 27). Invariably, these studies have analyzedthe behavior of the RAG proteins as part of a DNA-protein complex.Since we and others have shown that the RAG proteins can bindDNA in specific and nonspecific manners (1, 15, 25), itwas not initially clear to us whether protein-protein interactionsindependent of protein-DNA interactions play a role in the complexformation. For example, in the most extreme case, each proteincould be present in the complex purely through its contact withDNA. We undertook this study from the perspective that a descriptionof the simpler protein-protein interactions and stoichiometrieswith and without single RSS-containing DNA molecules would giveus a better understanding of the components available for futurestudies of the more complicated structure containing twoRSSs.

The DNA recombination occurs through a cutting and pasting mechanism in which specific double-strand breaks are generatedadjacent to each RSS (13). This cleavage reaction occurs intwo steps. First, one DNA strand is nicked at the coding sequencebordering the heptamer. This nick is then converted to a double-strandbreak in a second step that leaves the so-called signal end asblunt duplex DNA and the coding end as an unusual DNA hairpin(13). Since the coding DNA is no longer covalently bound tothe RSS, it remains something of a mystery as to how the two codingends are held in proximity during the interval of processing beforethey are ultimately joined together. The cleaved coding end hasbeen found retained within a synaptic complex (7), and we reporthere that the coding end liberated by DNA cleavage of a singleRSS is retained by a complex containing the RAGproteins.

Central to the cleavage steps are the two proteins RAG1 and RAG2 (16, 22). Most significantly, these two proteins aresufficient to reconstitute site-specific cleavage of DNA substratesin vitro. It appears that the two proteins cooperate at everystage for which an activity can be measured. While DNA bindingcan be demonstrated for RAG1 (4, 23) and weakly for RAG2(15), the specificity of binding for the RSS is enhanced whenboth proteins are present simultaneously (1, 15, 25). Furthermore,nicking and hairpin formation on either duplex DNA substratesor prenicked substrates proceeds only in the presence of bothproteins (13, 28, 29), and hairpin opening may also be mediatedby both proteins (2).

Coupled cleavage of substrates that contain the correct pair of RSS elements can also be observed with RAG1 and RAG2, as demonstratedwith purified proteins (30), and with cell extracts (5),though it is enhanced by the additional presence of the DNA bendingprotein HMG1 (27). The cleavage activities show a dependenceon divalent cations. Cleavage of individual RSS-containing oligonucleotidesis obtained only in the presence of manganese, while coupled cleavagecan be obtained with the more physiologic magnesium ion. The behaviorof coupled cleavage supports the existence of a biochemical intermediatein which both RSSs are bound prior to either being cleaved. TwoRSS elements can be bound simultaneously by RAG1 and RAG2 in amanner that follows the 12/23 rule (7). This synaptic structureis similar in principle to reaction intermediates already studiedin greater detail during bacterial recombination and transpositionreactions (for example, reference 10. There is evidence thatthe natural cleavage reaction within cells proceeds through acoupled cleavage pathway, supporting the idea that a synapticcomplex of proteins and DNA is the biologically relevant process(24). Such a structure requires protein-DNA binding within thesingle RSS and additional binding events to bridge the two RSSs.Better understanding of these events requires an appreciationof the protein-protein and protein-DNA interactions availableto the RAG proteins. This is the major subject of thisreport.

The natural RAG1 and RAG2 proteins of mice contain 1,040 and 527 amino acid residues, respectively. The full-length proteinsare difficult to obtain in biochemically useful quantities owingto their marginal solubilities when overexpressed. Fortunately,truncated core regions of these proteins maintain all currentlymeasurable activities and are capable of executing the completereaction in cells with normalfidelity.

The biochemistry of the cleavage reaction has been studied by means of the expression and purification of these truncatedvariants, usually in the form of a fusion protein (13), andwe used the same reagents in this study. The N-terminal regionof the full-length RAG1 protein contains a region that has theattributes of a ring finger domain and has been expressed andsubjected to structural analysis (18). This domain is capableof serving as a dimerization domain in isolation. However, itis absent in the functional truncated version of RAG1 used inthis study. It follows that the homodimerization of RAG1 and theadditional protein-protein interactions in the tetrameric complexmust be mediated by sequences within the coreregions.

To characterize the interactions that can occur among these proteins and DNA, we have purified the core regions of these twoproteins, expressed as maltose binding protein fusions (calledMR1 and MR2), and analyzed the physical properties of these proteinsindividually, mixed together, and in the absence or presence ofDNA substrates. In the absence of DNA, gel filtration experimentsreveal that MR1 alone exists predominantly as a homodimer, RAG2alone has monomer, dimer, and higher forms, and coexpressed MR1and MR2 proteins form a mixed tetramer in solution which containstwo of eachsubunit.

DNA-protein complexes are visualized by an electrophoretic mobility shift assay (EMSA). While the individual proteins canbind to DNA, they are not active in DNA cleavage. The mixtureof both proteins bound to DNA forms two bands in EMSA, and weare able to purify these bands and demonstrate that only one isactive in cleaving the substrate. The molecular mass of this activeband is determined by Ferguson plot analysis (3, 12, 17)and found to correspond to the same tetramer of MR1 and MR2 plusone DNA molecule. Additionally, we show that cleavage of DNA insolution followed by EMSA reveals that both DNA products followingcleavage can still be held together in a stable protein-DNA complexwith the same mobility as the uncleaved DNA. These data suggestthat a tetramer of RAG proteins is the active form bound to asingle RSS in the V(D)J recombinationreaction.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Proteins. Baculovirus stocks for MR1 and MR2 (13) were obtained from Martin Gellert (National Institutes of Health). MR1 and MR2 arefusion proteins, each containing an N-terminal maltose bindingprotein followed by the functional core region of mouse RAG1 (residues384 to 1008) or RAG2 (residues 1 to 387) respectively. The C terminicarry a polyhistidine tag followed by three tandem copies of thec-Myc epitope tag as used previously (19). MR1 and MR2 proteinswere expressed individually or simultaneously by coinfection ofthe SF9 insect cell line. Proteins were harvested after 66 h ofinfection and purified on nitrilotriacetic acid-agarose (Qiagen)charged with Ni²⁺ as described elsewhere (28). Fractions containing the fusionproteins were pooled and loaded onto amylose resin (New EnglandBiolabs). The column was washed extensively with buffer A (20mM Tris-HCl [pH 7.4], 500 mM NaCl, 10 mM $beta$ -mercaptoethanol, 1mM EDTA) containing 0.2% Tween 20 followed by elution in bufferA plus 10 mM maltose. Protein-containing fractions were pooledand dialyzed against buffer R (25 mM Tris-HCl [pH 8.0], 150 mMKCl, 2 mM dithiothreitol, 10% glycerol) for 3 h. Aliquots werefrozen in liquid nitrogen and stored at $-$ 80°C.

Proteins purified through one chromatography step were 90% pure. Double-affinity-purified proteins were homogeneous on Coomassiebrilliant blue-stainedgels.

Gel exclusion chromatography. RAG proteins were loaded onto a Superdex 200 (16 mm by 60 cm) column (Amersham Pharmacia Biotech) and eluted with buffer R.Fractions were analyzed on a sodium dodecyl sulfate (SDS)-4 to12% polyacrylamide gel, blotted to nitrocellulose, and visualizedwith anti-Myc monoclonal antibody 9E10. Standard proteins wereloaded and developed in the same buffer system and then visualizedby Coomassie brilliant blue staining. Elution data were analyzedaccording to the formula K_av = (V_e $-$ V₀)/(V_t $-$ V₀). The totalvolume (V_t) of the column is 123 ml, and the void volume (V₀)of the column is 47 ml, as determined by blue dextran 2000. Fractionsof 2-ml volume werecollected.

DNA substrates. Oligonucleotides were synthesized with a Perceptive Biosystems 8909 synthesizer. All substrates were 5'-end labeled with [³²P]ATP, using T4 polynucleotide kinase (Amersham Pharmacia Biotech)as indicated. 12RSS (53 bp) and 23RSS (58 bp) oligonucleotidesused were M-1 (5'-GCAGGTCGACTTACACAGTGCTACAGACTGGAACAAAAACCCTCGAGGTCTCC-3')with its complement M-2 and M-20 (5'-GGGGATCCACTTACACAGTGGTAGTACTCCACTGTCTGGCTGTACAAAAACCACGCGT-3')with its complement M-22, respectively. Typically, one strandis labeled, annealed with its complement, purified by gel filtrationon an STE Select-D G-25 spin column (5Prime-3Prime), and elutedwith STE buffer (10 mM Tris-HCl, 100 mM NaCl, 1 mM EDTA [pH 8.0]).In early versions of the experiments, gel-purified double-strandedprobes yielded the same results. Subsequent experiments were performedwith a slight excess (5 to 10%) of the unlabeled strand in theannealing step to ensure that all of the labeled strand was inthe double-strand form. Gel analysis of the probe confirmed theabsence of single-strandedprobe.

Binding and EMSA. Binding mixtures (10 µl) contained 0.1 pmol of ³²P-labeled oligonucleotide substrate DNA in a mixture containing 60 mM imidazole(pH 7.0), 50 mM sodium acetate, 1 mM CaCl₂ (unless otherwise stated),2 mM dithiothreitol, bovine serum albumin (80 µg/ml), and 10%dimethyl sulfoxide (DMSO). RAG1 and RAG2 were added as indicated.Unless otherwise stated, reaction mixtures were incubated on icefor 20 min. To each mixture, 3 µl of gel loading dye (30% glycerol,0.01% bromphenol blue) was added, and samples were analyzed byelectrophoresis through 5% polyacrylamide gel, using an imidazolebuffer system (25 mM imidazole [pH 7.0], 0.05% Tween 20, 10% DMSO).EMSA gels were prerun for at least 30 min. Preliminary experimentsto test the effect of temperature on the stability of the EMSAcomplexes indicated that complexes run at ambient temperaturewere as stable as those run at 4°C; consequently, all experimentsdescribed here were performed at room temperature. ³²P-labeled DNA was detected by autoradiography using a MolecularDynamics PhosphorImager and ImageQuant (version 1.2)software.

Ferguson plot assay to determine the size of a protein-DNA complex was carried out with the same binding and electrophoresisconditions as used for the EMSA described above. A series of continuousgels (16 cm long) of differing total polyacrylamide concentrations(29:1 acrylamide:bisacrylamide) were cast and prerun for 30 minin imidazole buffer. Binding reaction mixtures with ³²P labeled DNA were loaded onto all four gels; 1 µg of each standardnative protein molecular weight marker (Sigma) was mixed withthe same loading buffer and run alongside the binding reactionsat 300 V. Lanes containing the binding reaction mixtures weresubjected to autoradiography, with the position of the bromophenolblue dye front marked. The remainder of the gels were stainedwith Coomassie blue. The distances migrated by the protein-DNAcomplexes and by each standard were then measured and dividedby the distance migrated by the bromophenol blue in the same sample,giving the relative mobility (R_f). Where the protein standardscontain more than one band due to the presence of charge isomers,the R_f of the major isomer was used. The data were analyzed asdescribed elsewhere (3, 12, 17).

Cleavage activity of the protein-DNA complexes. Binding reactions were assembled as described above, varying the divalent cation as indicated. Probe DNA was labeled on onestrand. Complexes were separated by EMSA and identified by autoradiographyof the wet gel. Appropriate bands were excised and incubated incleavage buffer containing the desired cation at 37°C. DNA wasrecovered from the gel slice following incubation by disassemblyof the complexes in SDS (0.1%, final concentration), with repeatedfreezes and centrifugation. The recovered DNA was analyzed bysubsequent electrophoresis through a 10% polyacrylamide gel, usinga Tris-borate-EDTA (TBE) buffer system. Products were detectedby autoradiography of the driedgel.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

RAG proteins in the absence of DNA. In characterizing the protein and DNA complexes active in V(D)J recombination, we used truncated forms of the RAG proteinsthat have been used in previous biochemical characterizations.Protein MR1 contains the core region of RAG1 (mouse residues 384to 1008) as part of a maltose binding protein fusion also containinga polyhistidine affinity tag and the c-Myc epitope tag. The resultingmolecule has a predicted mass of 120 kDa. The RAG2 core (residues1 to 387) was expressed the same way, with the predicted monomermass of 92 kDa for this protein(MR2).

These two proteins were initially expressed individually, purified, and analyzed by size exclusion chromatography; Fig. 1Aand B show Western blots of alternate fractions obtained. Recallthat in an analysis of this type, larger molecules elute in earlierfractions and smaller molecules appear later. MR1 alone separatedas a single major species with its elution peak centered aboutfraction 30. MR2 presented a more complicated pattern, with proteineluting throughout a wide span of the profile, with one distinctpeak in fraction 32 and a second peak in fraction 36. Additionalmaterial representing higher-order forms is also seen. The centerof the distribution of MR2 alone falls slightly above the MR2dimer position. Figure 1C shows the contrasting behavior obtainedwhen the two proteins were coexpressed and copurified, using theaffinity tags present on both proteins. The infection was deliberatelybiased to produce more MR2 than MR1. The resulting profile showsthat the majority of both proteins eluted together in fraction26. Additional MR2 continued to elute in later fractions. Thisresult suggests that both proteins are present together in a largercomplex than is predominant with either protein in isolation.The molecular weight of the various peaks is determined from acurve generated from protein standards and is shown in Fig. 1D.The MR1 peak in Fig. 1A corresponds to an apparent molecular massof 247 kDa. The two peaks seen with MR2 in isolation correspondto 183 and 102 kDa, respectively. The peak obtained with coexpressedproteins represents an apparent mass of 443 kDa. The theory ofsize exclusion chromatography predicts a linear relationship forthe standard curve, as used here. The actual situation may deviatefrom the theoretical since the standard proteins may not be perfectglobular structures completely free of chemical interaction withthe gel matrix. We have therefore also recalculated the standardcurve as a cubic polynomial fit (not shown). This increases thefit of the standards to the curve from a least-squares value of0.995 for the linear fit to a value of 0.999 for the polynomialfit. With this alternate standard curve, the peak from Fig. 1Cwould represent a slightly greater predicted mass of 459 kDa.The difference in calculation does not alter our interpretation.These data indicate that MR1 in isolation exists predominantlyas a dimer and MR2 alone exists as a mixture of monomer, dimer,and larger forms. The coexpressed proteins in contrast form adistinct larger complex close to the expected mass of 426 kDaanticipated for two of each. The slightly larger than predictedmass, if significant, may represent an elongated shape for thetetrameric structure.

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FIG. 1. Gel filtration analysis of RAG proteins. (A to C) Western blots of alternate fractions collected by chromatography over Superdex 200 resin. (A) Purified MR1 (120-kDa monomer) shows a single peak. (B) Purified MR2 (92-kDa monomer) shows peaks in fractions 32 and 36 and additional higher forms. (C) Coexpressed and purified complex of MR1 plus MR2 shows a single peak which contains both proteins. (D) Calibration curve for protein standards (squares) and location of chromatogram peaks (circles). BSA, bovine serum albumin.

RAG proteins in the presence of DNA. We and others have previously shown that DNA-protein complexes can be assembled with various combinations of RAG proteinsand labeled oligonucleotide substrates (1, 2, 7, 15,25). These complexes can be visualized by EMSA. Figure 2 showsthe typical result of such an analysis. Here we show the behaviorof complexes formed on a 12RSS or 23RSS probe, with MR1 aloneor with coexpressed MR1 and MR2. In addition, this analysis wasperformed in the absence or presence of competitor dI-dC. Lane1 shows the MR1 alone assembling on a 12RSS probe in the absenceof dI-dC. Multiple bands can be seen extending up to the samplewell. Plotting of the mobilities of these bands from this or similargels indicates that they fall on an exponential curve, consistentwith a simple multimeric relationship between them (data not shown).A similar behavior occurs with a 23RSS DNA (lanes 2 and 3). Infact (data not shown), the same behavior can be obtained withunrelated DNA as a probe, suggesting that the bulk of the DNAbinding in this case is not sequence specific. The ability ofRAG1 to bind DNA nonspecifically has been reported before (1,15, 25). This point is reinforced by the behavior of the sameproteins and probes in the presence of dI-dC competitor (lanes7 to 9), where the higher-order bands disappear. In contrast,when both proteins are present (lanes 4 to 6 and 10 to 12), anew band which is resistant to competition appears. We and othershave shown that the lower band contains only RAG1 protein plusDNA, while the upper band contains both RAG1 and RAG2 (1, 15,25). This experiment was performed with the protein mixtureanalyzed in Fig. 1C, in which MR1 is fully associated in the tetramericform prior to the addition of the DNA. Despite effort to overrepresentthe MR2 in the mixture, the lower band persists, suggesting thatthe MR2 protein can be displaced from the preexisting MR1-MR2tetramer. It is not clear from our data if the bottom band representsMR1 originally present in a tetramer of MR1 and MR2 that spontaneouslydissociated prior to DNA binding. Alternatively, the binding toDNA or subsequent steps may destabilize the interaction of MR1to MR2, allowing some loss of MR2 from the tetramer. We hope toaddress this issue in future experiments. We have previously foundthat the binding of MR2 alone to DNA is very weak and is easilycompeted with dI-dC (15). Others, using different conditions,detected no binding (4, 23, 25). Consequently, we feelthat the important interactions involving RAG2 occur in the presenceof RAG1, and we have not pursued the description of the MR2 aloneon DNA.

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FIG. 2. EMSA analysis of protein binding to DNA. The two probes 12RSS (lanes 1, 4, 9, and 12) and 23RSS (lanes 2, 3, 5 to 8, 10, and 11) show equivalent behavior. MR1 alone or coexpressed MR1 and MR2 are bound in the absence (lanes 1 to 6) or presence (lanes 7 to 12) of competitor dI-dC. Protein binding to the 23RSS was performed at two concentrations. MR1 alone in the absence of dI-dC forms multiple bands. One band (marked) is unique to lanes that contain MR1 plus MR2.

Since the composition and stoichiometry of the protein complex on DNA are more relevant to the V(D)J recombination mechanismthan the behavior of the purified proteins themselves, we usedFerguson plot analysis to determine the molecular weight of thecomplexes visualized byEMSA.

In EMSA analysis, the mobility of the complex under native conditions is a complicated product of size, shape, charge andother forces such as interaction with the gel matrix. As a result,one cannot assume that the relative mobilities of different bandsin a single gel are direct reflections of the masses of theircomponents. The principle behind Ferguson plot analysis is thatby using a series of gels in all ways identical except for theconcentration of acrylamide, one can isolate the sieving propertiesof the gels from all other forces, which remain constant. Thechange in mobility of the complex as a function of change in acrylamideconcentration turns out to be directly proportional to the molecularradius of the particles being analyzed. This in turn is relatedexponentially to the molecular mass, given the simplifying assumptionof a globular structure. For the purposes of determining the stoichiometryof a complex, this assumption is not dangerous since the differencein mobility of a monomer versus a dimer is much more dramaticthan the nonlinearity introduced by a consideration of shape.This technique was originally applied to pure protein electrophoresis,but several studies have successfully used it to characterizethe masses of protein-DNA complexes (3, 12, 17).

Figure 3A shows the change in mobilities obtained in a series of gels for complexes that form on the 12RSS probe with MR1alone or in the presence of MR2. As the acrylamide concentrationincreases, the equivalent bands migrate more slowly, as shownby the connecting lines. Similar gels are run for each of thestandards (data not shown). For each family of bands, a plot ofthe log of the relative mobility versus acrylamide concentrationfalls on a line (Fig. 3B), the slope of which is proportionalto molecular radius. Small proteins sieve easily in all the gelsand do not exhibit a large change in mobility, while large proteinsare more sensitive to pore size and show a steeper slope. Thisallows one to construct a standard curve by using markers of knownmass (Fig. 3C). The slopes obtained for the complexes of MR1 orMR1 plus MR2 with DNA can then be transformed into an apparentmolecular mass by using the standard curve. In this analysis,the lowest bands formed by MR1 alone and the lower band formedin the presence of MR2 gave the same mass, 295 kDa. This is ingood accord with the expected mass of 275 kDa for a complex composedof two MR1 molecules (120 kDa each) plus one probe DNA molecule(35 kDa). This result confirms the interpretation of previousauthors (1, 15, 25) that the EMSA bands obtained with MR1alone and the comigrating band obtained in the presence of bothproteins contain only MR1. We add to this observation the appreciationthat it is actually a dimer of MR1 present within this complex.Similarly, the upper band obtained with both RAG proteins hasalready been shown to contain both proteins (25). We have previouslyshown that this band excised from the gel apparently containsan equal molar ratio of the two (15). Here we have shown thatthe mass of the complex is most consistent with a tetramer ofprotein on DNA. Given our previous result that the stoichiometryis equal, we conclude that there are two molecules of each proteinper complex. Purely on the basis of this mass estimate, we cannotrule out the possibility of two DNA molecules being present inthis complex, but the interpretation of one DNA molecule is mostconsistent with other experiments (see Discussion). The complexknown to contain both MR1 and MR2 (second from the bottom in Fig.3A) by this analysis yielded an apparent mass of 464 kDa. Thisis strikingly close to the predicted mass of 459 kDa for a tetramerof two MR1 molecules plus two MR2 molecules and one probe DNAmolecule. The higher-order bands visible in the MR1-only gelsare more difficult to size with certainty, as their slower migrationleads to a larger consequence of measurement errors. Our calculationsare consistent with the interpretation that these represent progressivemultimers of MR1 dimers on a single DNA molecule. Overall, theseexperiments demonstrate that MR1 binds to DNA as a dimer, andwhen MR2 is present, the stable complex with DNA contains twoof each protein.

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FIG. 3. Ferguson plot analysis of RAG protein-DNA complexes. (A) Isolated lanes from EMSA gels show the change in mobility of the native protein-DNA complexes in gels that differ solely in acrylamide concentration (indicated). Bands that represent the same complex under different gel conditions are linked by lines. Binding reactions were assembled in the absence of dI-dC competitor. The mathematical treatment of migration normalizes each lane to the migration of the dye front, thereby correcting for slight differences in runs between gels. (B) Calculation of the characteristic slopes. Migration data as in panel A for the standard proteins and selected experimental bands are plotted as a function of gel concentration. The y axis shows mobility calculated according to the formula y = 100 [log (R_f * 100)]. The relationship between migration and gel concentration is exponential, so the semilog plot yields a line. R_f represents the absolute migration divided by the migration of the dye front for that gel. Each line is described by the formula y = mx + b, where m is the slope. BSA, bovine serum albumin. (C) Ferguson plot. The inverse of the slope is directly proportional to the molecular radius of the particle, which in turn is directly proportional to mass for globular particles. Standards (squares) are plotted, and experimental samples (circles) are interpreted from the resulting standard curve.

Cleavage activity of the tetramer complex. Our results indicate that RAG1 and RAG2 can form a tetrameric complex in the absence or the presence of DNA. We wished todetermine whether that form was the only form capable of carryingout the cleavage reaction. One complication to experiments performedin solution is that reassortment of the components can occur.Even with complexes assembled under conditions of MR2 excess,we find that a band representing a species containing MR1 aloneappears in the EMSA gels. This finding suggests that MR2 bindswith sufficient weakness to disassociate from the protein-DNAcomplex. We therefore attempted the cleavage reaction within agel slice in which the individual complexes had already been separatedfrom each other. Figure 4A shows a representation of the probesused in the following assays. The duplex oligonucleotide containsa 12RSS and can be 5'-end labeled on either the top or bottomstrand as drawn. In an initial experiment, probe labeled on thebottom strand was used (Fig. 4B). The expected labeled productof the cleavage reaction would be the 40-bp signal end. Lane 1is a marker lane in which the cleavage reaction was performedin solution; lane 2 contains the probe alone. The remaining lanesrepresent complete reactions that were assembled on ice and thenseparated through a native gel to yield the two bands previouslyseen (as in Fig. 2, lane 12). These bands were identified, excisedfrom the gel, divided in two, and reincubated at the indicatedtemperature in the presence of reaction buffer. After 20 min,SDS was added to the gel slices, and the DNA was eluted and analyzedon another gel (Fig. 4B). As can be seen (lane 5), cleavage activitywas detected only in the band corresponding to the upper EMSAband incubated at 37°C. The identical sample maintained at 0°Cretained the original status (lane 6). This indicates that thecleavage truly occurred following the gel separation and not duringthe initial assembly of the reaction. Furthermore, the fasterEMSA band already shown to contain only MR1 was not active inthe cleavage assay (see below).

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FIG. 4. Cleavage assay applied to gel-purified bands. (A) Schematic representation of the two probes used for the assay. The 12RSS probe is represented by the triangle, with cleavage occurring at the heptamer border (vertical side) to produce the hairpinned coding end (13 bp) and signal end (40 bp). Only one of these products will be labeled, depending on which DNA strand is 5'-end labeled initially (asterisk). (B) Complexes assembled on ice in Mn²⁺ with both MR1 and MR2 were separated on a native gel, and the two bands were excised and incubated at the indicated temperature. The DNA was recovered and run in a second gel in TBE buffer. Lane M, marker of the cleavage reaction performed in solution; lane P, the unreacted probe. The excised band known to contain only the MR1 protein does not exhibit cleavage activity (lanes 3 and 4), but the excised band which contains both MR1 and MR2 (lanes 5 and 6) cleaves its DNA when incubated at 37°C. (C) Cleavage of probe in the excised MR1-MR2 band occurs only in Mn²⁺. Parallel reactions were assembled in Mg²⁺ and Mn²⁺ with 12RSS probes labeled individually on the top (T) or bottom (B) strand. A native gel was run, and the complexes containing MR1 plus MR2 were excised and then incubated in their original reaction buffer. The DNA was recovered and run in a gel in TBE buffer. Lanes 1 and 2 are cleavage reactions in solution for probes labeled on the top or bottom strand as markers. Activity on the probe labeled on the top (lanes 3 and 4) and bottom (lanes 5 and 6) strands is much stronger in the presence of Mn²⁺ than Mg²⁺.

In a more refined experiment (Fig. 4C), we concentrated entirely on the behavior of the complex containing tetrameric MR1plus MR2. Two probes were used, representing the 12RSS DNA labeleduniquely on the top or bottom strand. When the top strand is labeled,cleavage generates a 13-bp coding end, while the labeled bottomstrand is cleaved to form a 40-bp signal end. Again, the protein-DNAcomplexes were assembled in solution on ice and separated undernative conditions, and the band of interest was excised. In thisexperiment, parallel reactions were assembled in the presenceof Mg²⁺ or Mn²⁺. Reactions were performed with the top strand (lanes 1, 3, and4) or bottom strand (lanes 2, 5, and 6) labeled as probes; lanes1 and 2 are marker lanes in which cleavage was allowed to occurin solution. The MR1-MR2 complexes were isolated under EMSA conditions,excised, and then incubated in reaction buffer containing theoriginal metal ion. Signal ends and coding ends were generatedas previously found in solution. We find that cleavage occursprimarily in the Mn²⁺ lanes, yielding both expectedproducts.

We subsequently found (data not shown) that similar results could be obtained by assembling the initial reaction in the presenceof Ca²⁺ with later incubation in Mn²⁺ following gel separation, as previously shown for conventionalbinding and cleavage experiments (1, 8). Additional experimentswere performed with 23RSS probes equivalent to those shown. Weakercleavage was obtained with the same pattern as presented withthe 12RSS (data not shown). This is consistent with the knownpreference of the cleavage reaction for the 12RSS in the absenceof HMG1. Furthermore, experiments were also conducted in the presenceof both 12RSS and 23RSS simultaneously in the hopes that an additionalsynaptic complex could be identified (8) or to assess whetherthe presence of both DNA species would permit cleavage in thepresence of Mg²⁺. Neither result was obtained (data not shown), which we viewas additional evidence that this tetrameric protein complex isassembled on a single molecule of probeDNA.

The tetrameric complex retains both products following cleavage. A variation of this experiment produced an interesting result presented as Fig. 5. The same probes were used as in the previousexperiment, labeled individually on either the bottom (lanes 1to 3) or top (lanes 4 to 6) strand. The cleavage reaction wasassembled in solution with both MR1 and MR2 proteins in the presenceof Mn²⁺. This time the reaction was allowed to cleave the probe for 20min at 37°C. The reaction was separated by electrophoresis ona native gel, again producing the two bands previously characterized.Both bands were excised separately. The DNA within these bandswas extracted and analyzed in a second gel. Lanes 1 and 4 aremarker lanes cleaved in solution. DNA from the upper band, representingthe tetrameric MR1-MR2 complex, is shown in lanes 2 and 5; theDNA derived from the faster EMSA band which contains MR1 aloneis in lanes 3 and 6. Quantitation of the DNA in each lane indicatesthat approximately 30% of the cleaved signal is present in lanes2 and 50% is in lane 5 compared to the control lanes. Since partof the DNA is lost during the elution from the gel slice, we estimatethat at least 50% of the cleavage products are retained in thesecomplexes. We see that both cleaved signal-end and coding-endproducts were obtained from the tetrameric protein complex, whileno cleavage products were found in the MR1-only complex. It isapparent that following cleavage in solution, the tetrameric complexwas able to retain both signal and coding products. Furthermore,following cleavage the tetrameric complex is stable with respectto RAG2 binding since none of the cleaved complex was convertedinto the MR1-only form. Further analysis of the stability andinterconversions of these complexes is the subject of ongoinginvestigation in our laboratory. One important implication ofthis observation is that DNA-protein contacts must occur withinthe coding DNA outside the RSS. Retention of coding-end DNA followingcleavage has been previously observed in the study of synapticcomplexes (7). These contacts would permit the RAG proteinsto play additional roles in the subsequent processing and joiningstages of the recombination reaction.

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FIG. 5. Retention of both signal ends and coding ends in the MR1-MR2 complex. The same two probes used for Fig. 4 were assembled into cleavage reactions and incubated at 37°C. Complexes were separated in a native gel, and bands corresponding to MR1-MR2 complex (lanes 2 and 5) or the MR1-alone complex (lanes 3 and 6) were excised. DNA was recovered and run in a TBE gel. Lanes 1 and 4 are cleavage reactions in solution for probes labeled on the bottom or top strand as markers.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The V(D)J recombination reaction is believed to pass through a synaptic intermediate in which one 12RSS and one 23RSS arealigned prior to cleavage (7). The proteins RAG1 and RAG2,aided by the ubiquitous DNA bending protein HMG1, are sufficientto specify this pairing. A significant puzzle remains to determinethe structural basis by which these proteins interact differentlywith the two types of RSS and prefer to cleave complexes thatcontain one of each type over pairs of the same type of RSS. Ithas been argued that the 12/23 rule is enforced at the synapticstep (7) or subsequently at the stage of double-hairpin formation(31). We are addressing the challenge of understanding the fullcleavage reaction by first attempting to identify and characterizethe constituent protein-protein and protein-DNA interactions thatcontribute to the larger complex. Both RAG1 and RAG2 proteinsare known to be necessary for the site recognition (4, 23)and various cleavage steps (2, 9, 29). They can also bothbe found in a complex that can be identified by EMSA (1, 7,15, 25), and we report here that the EMSA complex is capableof cleaving the DNA; there has been no exploration of the stoichiometryor organization of protein and DNA in the complex. This functionalunit appears to be a tetramer composed of two molecules of eachRAG protein. In isolation the purified core region of RAG1, expressedas a fusion protein (MR1) with maltose binding protein, existspredominantly as a dimer. The fusion partner itself does not dimerize(New England Biolabs product literature). The RAG2 derivative(MR2) containing a functional core of that protein as a fusionconstruct also appears to form higher-order protein complexesin isolation. Monomer, dimer, and unresolved higher forms of MR2are all present in the gel exclusion chromatogram. More strikingis the analysis of the two proteins when coexpressed. We findthat a tetramer-sized complex containing both proteins is thedominant form in the absence of DNA. A complex containing RAG1and RAG2 has been identified previously in immunoprecipitatesof cell extracts (14). In this previous study, the two proteinsmay have been tethered by DNA derived from the cell rather thantruly representing a direct protein interaction. This concernis eliminated by using the highly purified proteins in thisstudy.

These results are extended by studies of the complexes that assemble on RSS-containing substrates. Previous reports indicatethat a mixture of RAG1 and RAG2 leads to two distinct complexesas revealed by EMSA (1, 15, 25). Using Ferguson plot analysis(3, 12, 17), we were able to determine that the faster-migratingcomplex behaves as a particle with molecular radius appropriatefor a dimer of MR1 on one molecule of the probe. The slower-migratingcomplex, in contrast, is known to contain both RAG1 and RAG2 (15,25) and in our analysis appears to be composed of the same tetrameras observed above plus one DNA molecule. This is consistent withour previous observation of apparent equimolar ratios of the twoproteins when this EMSA band was excised from the gel and analyzedby Western blotting (15). We are further able to show that onlythe EMSA band that contains both RAG1 and RAG2 derivatives iscapable of cleaving its DNA. The faster-migrating EMSA band containinga dimer of RAG1 derived from the same binding reaction does notcleave the DNA. This is additional evidence that RAG2 plays adirect role in the cleavage reaction rather than indirectly activatinga nuclease in RAG1. If RAG2 were able to operate transiently toactivate RAG1 in a hit-and-run manner, then the faster-migratingcomplex would be competent for cleavage since it has been exposedtoRAG2.

There is a logical difficulty posed by the cleavage of the coding DNA outside the RSS. Since the cleavage event occurs atthe border of the RSS, there is no basis for sequence-specificbinding to the adjacent coding DNA. Yet in the absence of binding,there would be nothing to prevent the newly cleaved hairpin-endedcoding DNA from separating from its future partner. We favor theargument that the RAG proteins exhibit both sequence-specificand nonspecific binding behaviors. While sequence-specific bindingis required to position the proteins at the heptamer and nonamer,nonspecific binding is required to position additional proteinat the coding DNA flanking the RSS. The tetrameric protein complexwould permit this by coordinating binding to the RSS and the codingflank. Persistent binding to the coding flank would retain thathairpinned product for furtherprocessing.

We have observed that both cleaved products are retained in the EMSA complex containing RAG1 and RAG2. Others have not detectedthe same phenomenon in EMSAs using different experimental conditions(1, 8). Our studies use conditions that differ from thoseused in the cited studies and have been optimized so that chemicalcross-linking is not necessary to maintain the integrity of thecomplex. A significant experimental difference is the inclusionof 10% DMSO in the native gels and electrophoresis buffer. Thepresence of DMSO in the binding reaction is now standard (1,8, 15, 25), and we feel that it helps stabilize the proteinsand prevent aggregation. We added a nonionic detergent for thesame reason. We also note that using imidazole as a pH bufferand lowering the pH to 7.0 reduces the likelihood of the polyhistidinetags interacting with each other through a bridging metal ion.Retention of the coding end was observed in the analysis of synapticcomplexes in a biotin pull-down assay (7). Our observationrepresents an extension of that finding, using a different systemin which there is no possibility that a larger aggregate couldentrap the coding DNAproduct.

In trying to appreciate the role of the protein tetramer identified in this report in the normal biochemistry of the recombinationreaction, it is important to be certain of the DNA content withinthis complex. At least two possibilities are consistent with ourdata. The tetrameric complex identified here might represent exactlyhalf of the synaptic complex. Additional protein-protein interactionswould hold together two tetramers, each carrying one RSS. The12/23 rule would act either at the level of stabilizing the assemblyof that larger complex or at a subsequent chemical step. Alternatively,the protein tetramer may possess sufficient binding capacity toincorporate two RSS-containing DNA molecules. We believe thatthe complexes examined in this study contain only one DNA molecule.The evidence is indirect, and we are pursuing the question. Insupport of our interpretation are the following data. First, theanalysis in Fig. 3 yields a mass for the complex close to thetheoretical mass of a tetramer plus one DNA molecule. Second,the conditions that we used in this assay do not include HMG1protein. This is significant because previous work (7) indicatesthat a significant paired complex containing two DNA moleculeswas obtained only in the presence of that protein. Third, ourresult of cleavage performed on gel-purified complexes shows preferredcleavage in the presence of Mn²⁺ over Mg²⁺ ions. We have attempted to perform the same experiment with mixturesof 12RSS and 23RSS DNAs (data not presented). Creation of pairedcomplexes should exhibit equivalent cleavage with both ions; however,this was not observed, indicating that the complexes that we examineddid not contain bothDNAs.

We know that there are contacts between RAG1 at both the heptamer and nonamer (15) (though not necessarily the same monomerof RAG1) and indirect evidence that RAG1 interacts with the codingflank (20). This leads us to favor the proposal that two proteintetramers would be required to form the synaptic structure, sincebinding to the heptamer, the nonamer, and the coding flank probablyoccupies more than half of the binding sites available in onetetramer, leaving too few additional binding sites for a symmetricinteraction with a secondRSS.

	ACKNOWLEDGMENT

This work was supported by NIH grant AI41711 to M.J.S.

	FOOTNOTES

^* Corresponding author. Mailing address: Medical College of Georgia, Institute of Molecular Medicine and Genetics, Program ofGene Regulation, CB-2803, Augusta, GA 30912-2650. Phone: (706)721-8761. Fax: (706) 721-8752. E-mail: moshe{at}immag.mcg.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Akamatsu, Y., and M. A. Oettinger. 1998. Distinct roles of RAG1 and RAG2 in binding the V(D)J recombination signal sequences. Mol. Cell. Biol. 18:4670-4678[Abstract/Free Full Text].

2. Besmer, E., J. Mansilla-Soto, S. Cassard, D. J. Sawchuk, G. Brown, M. Sadofsky, S. M. Lewis, M. C. Nussenzweig, and P. Cortes. 1998. Hairpin coding end opening is mediated by RAG1 and RAG2 proteins. Mol. Cell 2:817-828[Medline].

3. Bullock, B. P., and J. F. Habener. 1998. Phosphorylation of the cAMP response element binding protein CREB by cAMP-dependent protein kinase A and glycogen synthase kinase-3 alters DNA-binding affinity, conformation, and increases net charge. Biochemistry 37:3795-3809[Medline].

4. Difilippantonio, M. J., C. J. McMahan, Q. M. Eastman, E. Spanopoulou, and D. G. Schatz. 1996. RAG1 mediates signal sequence recognition and recruitment of RAG2 in V(D)J recombination. Cell 87:253-262[Medline].

5. Eastman, Q. M., T. M. J. Leu, and D. G. Schatz. 1996. Initiation of V(D)J recombination in-vitro obeying the 12/23-rule. Nature 380:85-88[Medline].

6. Gellert, M. 1997. Recent advances in understanding V(D)J recombination. Adv. Immunol. 64:39-64[Medline].

7. Hiom, K., and M. Gellert. 1998. Assembly of a 12/23 paired signal complex: a critical control point in V(D)J recombination. Mol. Cell 1:1011-1019[Medline].

8. Hiom, K., and M. Gellert. 1997. A stable RAG1-RAG2-DNA complex that is active in V(D)J cleavage. Cell 88:65-72[Medline].

9. Kim, D. R., and M. A. Oettinger. 1998. Functional analysis of coordinated cleavage in V(D)J recombination. Mol. Cell. Biol. 18:4679-4688[Abstract/Free Full Text].

10. Lavoie, B. D., and G. Chaconas. 1996. Transposition of phage Mu DNA. Curr. Top. Microbiol. Immunol. 204:83-102[Medline].

11. Lewis, S. M. 1994. The mechanism of V(D)J joining: lessons from molecular, immunological, and comparative analyses. Adv. Immunol. 56:27-150[Medline].

12. May, G., C. Sutton, and H. Gould. 1991. Purification and characterization of Ku-2, an octamer-binding protein related to the autoantigen Ku. J. Biol. Chem. 266:3052-3059[Abstract/Free Full Text].

13. McBlane, J. F., D. C. van Gent, D. A. Ramsden, C. Romeo, C. A. Cuomo, M. Gellert, and M. A. Oettinger. 1995. Cleavage at a V(D)J recombination signal requires only RAG1 and RAG2 proteins and occurs in two steps. Cell 83:387-395[Medline].

14. McMahan, C. J., M. J. Sadofsky, and D. G. Schatz. 1997. Definition of a large region of RAG1 that is important for coimmunoprecipitation of RAG2. J. Immunol. 158:2202-2210[Abstract].

15. Mo, X., B. Tu, and M. Sadofsky. 1999. RAG1 and RAG2 cooperate in specific binding to the recombination signal sequence in vitro. J. Biol. Chem. 274:7025-7032[Abstract/Free Full Text].

16. Oettinger, M. A., D. G. Schatz, C. Gorka, and D. Baltimore. 1990. RAG-1 and RAG-2, adjacent genes that synergistically activate V(D)J recombination. Science 248:1517-1523[Abstract/Free Full Text].

17. Orchard, K., and G. E. May. 1993. An EMSA-based method for determining the molecular weight of a protein-DNA complex. Nucleic Acids Res. 21:3335-3336[Free Full Text].

18. Rodgers, K. K., Z. Bu, K. G. Fleming, D. G. Schatz, D. M. Engelman, and J. E. Coleman. 1996. A zinc-binding domain involved in the dimerization of RAG1. J. Mol. Biol. 260:70-84[Medline].

19. Sadofsky, M. J., J. E. Hesse, J. F. McBlane, and M. Gellert. 1993. Expression and V(D)J recombination activity of mutated RAG-1 proteins. Nucleic Acids Res. 21:5644-5650[Abstract/Free Full Text].

20. Sadofsky, M. J., J. E. Hesse, D. C. van Gent, and M. Gellert. 1995. RAG-1 mutations that affect the target specificity of V(D)J recombination: a possible direct role of RAG-1 in site recognition. Genes Dev. 9:2193-2199[Abstract/Free Full Text].

21. Sawchuk, D. J., F. Weis-Garcia, S. Malik, E. Besmer, M. Bustin, M. C. Nussenzweig, and P. Cortes. 1997. V(D)J recombination: modulation of RAG1 and RAG2 cleavage activity on 12/23 substrates by whole cell extract and DNA-bending proteins. J. Exp. Med. 185:2025-2032[Abstract/Free Full Text].

22. Schatz, D. G., M. A. Oettinger, and D. Baltimore. 1989. The V(D)J recombination activating gene, RAG-1. Cell 59:1035-1048[Medline].

23. Spanopoulou, E., F. Zaitseva, F. Wang, S. Santagata, D. Baltimore, and G. Panayotou. 1996. The homeodomain region of Rag-1 reveals the parallel mechanisms of bacterial and V(D)J recombination. Cell 87:263-276[Medline].

24. Steen, S. B., L. Gomelsky, S. L. Speidel, and D. B. Roth. 1997. Initiation of V(D)J recombination in vivo: role of recombination signal sequences in formation of single and paired double-strand breaks. EMBO J. 16:2656-2664[Medline].

25. Swanson, P. C., and S. Desiderio. 1998. V(D)J recombination signal recognition: distinct, overlapping DNA-protein contacts in complexes containing RAG1 with and without RAG2. Immunity 9:115-125[Medline].

26. Tonegawa, S. 1983. Somatic generation of antibody diversity. Nature 302:575-581[Medline].

27. van Gent, D. C., K. Hiom, T. T. Paull, and M. Gellert. 1997. Stimulation of V(D)J cleavage by high mobility group proteins. EMBO J. 16:2665-2670[Medline].

28. van Gent, D. C., J. F. McBlane, D. A. Ramsden, M. J. Sadofsky, J. E. Hesse, and M. Gellert. 1995. Initiation of V(D)J recombination in a cell-free system. Cell 81:925-934[Medline].

29. van Gent, D. C., K. Mizuuchi, and M. Gellert. 1996. Similarities between initiation of V(D)J recombination and retroviral integration. Science 271:1592-1594[Abstract].

30. van Gent, D. C., D. A. Ramsden, and M. Gellert. 1996. The Rag1 and Rag2 proteins establish the 12/23-rule in V(D)J recombination. Cell 85:107-113[Medline].

31. West, R. B., and M. R. Lieber. 1998. The RAG-HMG1 complex enforces the 12/23 rule of V(D)J recombination specifically at the double-hairpin formation step. Mol. Cell. Biol. 18:6408-6415[Abstract/Free Full Text].

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1.	Akamatsu, Y., and M. A. Oettinger. 1998. Distinct roles of RAG1 and RAG2 in binding the V(D)J recombination signal sequences. Mol. Cell. Biol. 18:4670-4678[Abstract/Free Full Text].
2.	Besmer, E., J. Mansilla-Soto, S. Cassard, D. J. Sawchuk, G. Brown, M. Sadofsky, S. M. Lewis, M. C. Nussenzweig, and P. Cortes. 1998. Hairpin coding end opening is mediated by RAG1 and RAG2 proteins. Mol. Cell 2:817-828[Medline].
3.	Bullock, B. P., and J. F. Habener. 1998. Phosphorylation of the cAMP response element binding protein CREB by cAMP-dependent protein kinase A and glycogen synthase kinase-3 alters DNA-binding affinity, conformation, and increases net charge. Biochemistry 37:3795-3809[Medline].
4.	Difilippantonio, M. J., C. J. McMahan, Q. M. Eastman, E. Spanopoulou, and D. G. Schatz. 1996. RAG1 mediates signal sequence recognition and recruitment of RAG2 in V(D)J recombination. Cell 87:253-262[Medline].
5.	Eastman, Q. M., T. M. J. Leu, and D. G. Schatz. 1996. Initiation of V(D)J recombination in-vitro obeying the 12/23-rule. Nature 380:85-88[Medline].
6.	Gellert, M. 1997. Recent advances in understanding V(D)J recombination. Adv. Immunol. 64:39-64[Medline].
7.	Hiom, K., and M. Gellert. 1998. Assembly of a 12/23 paired signal complex: a critical control point in V(D)J recombination. Mol. Cell 1:1011-1019[Medline].
8.	Hiom, K., and M. Gellert. 1997. A stable RAG1-RAG2-DNA complex that is active in V(D)J cleavage. Cell 88:65-72[Medline].
9.	Kim, D. R., and M. A. Oettinger. 1998. Functional analysis of coordinated cleavage in V(D)J recombination. Mol. Cell. Biol. 18:4679-4688[Abstract/Free Full Text].
10.	Lavoie, B. D., and G. Chaconas. 1996. Transposition of phage Mu DNA. Curr. Top. Microbiol. Immunol. 204:83-102[Medline].
11.	Lewis, S. M. 1994. The mechanism of V(D)J joining: lessons from molecular, immunological, and comparative analyses. Adv. Immunol. 56:27-150[Medline].
12.	May, G., C. Sutton, and H. Gould. 1991. Purification and characterization of Ku-2, an octamer-binding protein related to the autoantigen Ku. J. Biol. Chem. 266:3052-3059[Abstract/Free Full Text].
13.	McBlane, J. F., D. C. van Gent, D. A. Ramsden, C. Romeo, C. A. Cuomo, M. Gellert, and M. A. Oettinger. 1995. Cleavage at a V(D)J recombination signal requires only RAG1 and RAG2 proteins and occurs in two steps. Cell 83:387-395[Medline].
14.	McMahan, C. J., M. J. Sadofsky, and D. G. Schatz. 1997. Definition of a large region of RAG1 that is important for coimmunoprecipitation of RAG2. J. Immunol. 158:2202-2210[Abstract].
15.	Mo, X., B. Tu, and M. Sadofsky. 1999. RAG1 and RAG2 cooperate in specific binding to the recombination signal sequence in vitro. J. Biol. Chem. 274:7025-7032[Abstract/Free Full Text].
16.	Oettinger, M. A., D. G. Schatz, C. Gorka, and D. Baltimore. 1990. RAG-1 and RAG-2, adjacent genes that synergistically activate V(D)J recombination. Science 248:1517-1523[Abstract/Free Full Text].
17.	Orchard, K., and G. E. May. 1993. An EMSA-based method for determining the molecular weight of a protein-DNA complex. Nucleic Acids Res. 21:3335-3336[Free Full Text].
18.	Rodgers, K. K., Z. Bu, K. G. Fleming, D. G. Schatz, D. M. Engelman, and J. E. Coleman. 1996. A zinc-binding domain involved in the dimerization of RAG1. J. Mol. Biol. 260:70-84[Medline].
19.	Sadofsky, M. J., J. E. Hesse, J. F. McBlane, and M. Gellert. 1993. Expression and V(D)J recombination activity of mutated RAG-1 proteins. Nucleic Acids Res. 21:5644-5650[Abstract/Free Full Text].
20.	Sadofsky, M. J., J. E. Hesse, D. C. van Gent, and M. Gellert. 1995. RAG-1 mutations that affect the target specificity of V(D)J recombination: a possible direct role of RAG-1 in site recognition. Genes Dev. 9:2193-2199[Abstract/Free Full Text].
21.	Sawchuk, D. J., F. Weis-Garcia, S. Malik, E. Besmer, M. Bustin, M. C. Nussenzweig, and P. Cortes. 1997. V(D)J recombination: modulation of RAG1 and RAG2 cleavage activity on 12/23 substrates by whole cell extract and DNA-bending proteins. J. Exp. Med. 185:2025-2032[Abstract/Free Full Text].
22.	Schatz, D. G., M. A. Oettinger, and D. Baltimore. 1989. The V(D)J recombination activating gene, RAG-1. Cell 59:1035-1048[Medline].
23.	Spanopoulou, E., F. Zaitseva, F. Wang, S. Santagata, D. Baltimore, and G. Panayotou. 1996. The homeodomain region of Rag-1 reveals the parallel mechanisms of bacterial and V(D)J recombination. Cell 87:263-276[Medline].
24.	Steen, S. B., L. Gomelsky, S. L. Speidel, and D. B. Roth. 1997. Initiation of V(D)J recombination in vivo: role of recombination signal sequences in formation of single and paired double-strand breaks. EMBO J. 16:2656-2664[Medline].
25.	Swanson, P. C., and S. Desiderio. 1998. V(D)J recombination signal recognition: distinct, overlapping DNA-protein contacts in complexes containing RAG1 with and without RAG2. Immunity 9:115-125[Medline].
26.	Tonegawa, S. 1983. Somatic generation of antibody diversity. Nature 302:575-581[Medline].
27.	van Gent, D. C., K. Hiom, T. T. Paull, and M. Gellert. 1997. Stimulation of V(D)J cleavage by high mobility group proteins. EMBO J. 16:2665-2670[Medline].
28.	van Gent, D. C., J. F. McBlane, D. A. Ramsden, M. J. Sadofsky, J. E. Hesse, and M. Gellert. 1995. Initiation of V(D)J recombination in a cell-free system. Cell 81:925-934[Medline].
29.	van Gent, D. C., K. Mizuuchi, and M. Gellert. 1996. Similarities between initiation of V(D)J recombination and retroviral integration. Science 271:1592-1594[Abstract].
30.	van Gent, D. C., D. A. Ramsden, and M. Gellert. 1996. The Rag1 and Rag2 proteins establish the 12/23-rule in V(D)J recombination. Cell 85:107-113[Medline].
31.	West, R. B., and M. R. Lieber. 1998. The RAG-HMG1 complex enforces the 12/23 rule of V(D)J recombination specifically at the double-hairpin formation step. Mol. Cell. Biol. 18:6408-6415[Abstract/Free Full Text].