Rentiation and proliferation of DN3 thymocytes as they transition from DN3E to DN3L, despite intact TCRb expression. Additionally, the DN to DP transition in 1KO and DKO mice was reduced. Of note, we found that despite PD168393 showing elevated frequencies of DN4 cd T cells, RasGRP1 and/or RasGRP3 does not appear to regulate ab vs cd lineage commitment. Finally, we found that 1KO and DKO DN3 thymocytes were defective in ERK activation following SDF1a stimulation, which may contribute to impaired b-selection. Our findings provide a basis for understanding RasGRP mediated control of the b-selection checkpoint and the downstream consequences of inefficient RasGRP-mediated Ras activation during thymopoiesis. In most cases, RasGRP1 and RasGRP1/3-deficient thymocytes displayed equivalent deficiencies in b-selection, while 3KO mice were mostly normal. Therefore, we attribute most of the deficiencies in b-selection observed in DKO mice to a loss of RasGRP1 and suggest that RasGRP3 cannot compensate for the loss of RasGRP1. Indeed, it has been shown that RasGRP1 is the most highly expressed RasGRP member in DN3a thymocytes [34]. The lack of a difference between RasGRP1 KO and RasGRP1/3 DKO mice contrasts the finding of the Zhang group where RasGRP4-defient mice showed no impairment in bselection, but the combined loss of RasGRP1 and 4 showed a more profound phenotype than RasGRP1 deficiency alone. This suggests that RasGRP4 could compensate somewhat for the loss of RasGRP1 [24]. The difference observed between RasGRP1/ 3 DKO and RasGRP1/4 DKO is likely due to relatively higher expression of RasGRP4 than RasGRP3 in DN3 thymocytes as reported by the Immunological Genome Project [24,34]. The development of DN into DP is a complex multi-stage program involving interactions between developing thymocytes and the diverse elements that make up the thymic microenvironment. RasGRP1 ablation results in inefficient development of DN into DP (Fig. 2b). Signaling downstream of the K162 web pre-TCR is known to involve the signaling molecules Zap70, Syk, LAT and SLP76, as well as activation of the Ras/ERK signaling pathway [5?0].RasGRP1 Is Required for b-SelectionFigure 6. RasGRP1 KO, RasGRP3 KO and RasGRP1/3 DKO thymocytes show intact survival. Percentages of DN3 (CD42CD82Thy1.2+CD442CD25+), DN4 (CD42CD82Thy1.2+CD442CD252) and DP (CD4+CD8+Thy1.2+) showing active caspase 3. doi:10.1371/journal.pone.0053300.gGiven that RasGRP1 contains a physiologically relevant C1 domain that binds DAG, it is likely that LAT mediated PLCc recruitment, activation and subsequent DAG production in response to pre-TCR signaling recruits RasGRP1 to the plasma membrane, resulting in Ras activation [2,35]. In support of this mode of RasGRP1 regulation, although not extensively studied, mice with a LAT Y136F mutation that abrogates PLCc recruitment and activation show impaired DN to DP development, suggesting impaired b-selection [36,37]. However, RasGRP1 regulation downstream of the pre-TCR remains poorly understood. We have identified a novel role for RasGRP1 downstream of CXCR4 activation in DN3 thymocytes. RasGRP1 deficient DN3 cells are unable to activate ERK in response to SDF1a stimulation of CXCR4. However, RasGRP1 deficient DN3 are able to activate AKT downstream of CXCR4 activation. Interestingly, CXCR4 deficient thymi show impaired b-selection and signals transduced through CXCR4 are important during early T cell development [12]. The mechanism of RasGRP1 activation downstream of CXCR4 remain.Rentiation and proliferation of DN3 thymocytes as they transition from DN3E to DN3L, despite intact TCRb expression. Additionally, the DN to DP transition in 1KO and DKO mice was reduced. Of note, we found that despite showing elevated frequencies of DN4 cd T cells, RasGRP1 and/or RasGRP3 does not appear to regulate ab vs cd lineage commitment. Finally, we found that 1KO and DKO DN3 thymocytes were defective in ERK activation following SDF1a stimulation, which may contribute to impaired b-selection. Our findings provide a basis for understanding RasGRP mediated control of the b-selection checkpoint and the downstream consequences of inefficient RasGRP-mediated Ras activation during thymopoiesis. In most cases, RasGRP1 and RasGRP1/3-deficient thymocytes displayed equivalent deficiencies in b-selection, while 3KO mice were mostly normal. Therefore, we attribute most of the deficiencies in b-selection observed in DKO mice to a loss of RasGRP1 and suggest that RasGRP3 cannot compensate for the loss of RasGRP1. Indeed, it has been shown that RasGRP1 is the most highly expressed RasGRP member in DN3a thymocytes [34]. The lack of a difference between RasGRP1 KO and RasGRP1/3 DKO mice contrasts the finding of the Zhang group where RasGRP4-defient mice showed no impairment in bselection, but the combined loss of RasGRP1 and 4 showed a more profound phenotype than RasGRP1 deficiency alone. This suggests that RasGRP4 could compensate somewhat for the loss of RasGRP1 [24]. The difference observed between RasGRP1/ 3 DKO and RasGRP1/4 DKO is likely due to relatively higher expression of RasGRP4 than RasGRP3 in DN3 thymocytes as reported by the Immunological Genome Project [24,34]. The development of DN into DP is a complex multi-stage program involving interactions between developing thymocytes and the diverse elements that make up the thymic microenvironment. RasGRP1 ablation results in inefficient development of DN into DP (Fig. 2b). Signaling downstream of the pre-TCR is known to involve the signaling molecules Zap70, Syk, LAT and SLP76, as well as activation of the Ras/ERK signaling pathway [5?0].RasGRP1 Is Required for b-SelectionFigure 6. RasGRP1 KO, RasGRP3 KO and RasGRP1/3 DKO thymocytes show intact survival. Percentages of DN3 (CD42CD82Thy1.2+CD442CD25+), DN4 (CD42CD82Thy1.2+CD442CD252) and DP (CD4+CD8+Thy1.2+) showing active caspase 3. doi:10.1371/journal.pone.0053300.gGiven that RasGRP1 contains a physiologically relevant C1 domain that binds DAG, it is likely that LAT mediated PLCc recruitment, activation and subsequent DAG production in response to pre-TCR signaling recruits RasGRP1 to the plasma membrane, resulting in Ras activation [2,35]. In support of this mode of RasGRP1 regulation, although not extensively studied, mice with a LAT Y136F mutation that abrogates PLCc recruitment and activation show impaired DN to DP development, suggesting impaired b-selection [36,37]. However, RasGRP1 regulation downstream of the pre-TCR remains poorly understood. We have identified a novel role for RasGRP1 downstream of CXCR4 activation in DN3 thymocytes. RasGRP1 deficient DN3 cells are unable to activate ERK in response to SDF1a stimulation of CXCR4. However, RasGRP1 deficient DN3 are able to activate AKT downstream of CXCR4 activation. Interestingly, CXCR4 deficient thymi show impaired b-selection and signals transduced through CXCR4 are important during early T cell development [12]. The mechanism of RasGRP1 activation downstream of CXCR4 remain.