He dried gel pieces were rehydrated with 20 mM DTT in 50 mM

September 25, 2017

He dried gel pieces were rehydrated with 20 mM DTT in 50 mM Ambic for 40 min at 56uC. Excess of reagent was removed and 55 mM iodoacetamide (IAA) in Ambic 50 mM was added for 30 min RT at dark. The remaining liquid was removed and washed out with 25 mM Ambic, followed by dehydration with ACN. After its removal, the gels were dried again. For digestion, dried gels were incubated with 10 ng/mL trypsin in 25 mM Ambic for 15 min (Trypsin Gold Mass spectrometry, Promega, Madison, USA). DMXAA chemical information Peptides were sequentially extracted from the gels initially in 50 ACN (v/v) with 5 formic acid for 14 h at 37uC, then in 50 ACN (v/v) with 1 formic acid for 15 min, followed by 60 methanol (v/v) with 1 formic acid for 15 min and twice with 100 ACN at 45uC under sonication (40kHz/30W, Branson, Danbury, USA). Extracts were dried using a vacuum concentrator (Eppendorf, Hamburg, Germany) and kept at -20uC. Prior to MS identification, dried peptides were dissolved in 12 mL 0.1 formic acid. The peptides were identified 18325633 and quantified by LC-ESI-Q-TOF MS (Liquid Chromatography Electrospray Ionization Quadrupole Time of Flight Mass Spectrometry) (Waters, Mildord, USA). MassLynx 4.1 SCN662 software (Waters, Mildord, USA) was used to submit the combined MS and MS/MS data to MASCOT database search engine (http://www.matrixscience.com) (version 2007.12.04) based on IPI (International Protein Index) protein database restricted to taxonomies Mus musculus (Mouse). The search was limited with a mass tolerance of 100 ppm and only one missed cleavage per peptide was allowed. For modification of peptides, cysteine carbamido-methylation (fixed) and methionine oxidation (variable) were considered. Significant matching proteinSample Preparation for 2DEKidney samples were homogenized using mortar and pestle in liquid nitrogen. Denaturation Compound C dihydrochloride web buffer (7 M urea, 2 M de thioureia, 4 CHAPS, 1 DTT and 0.5 IPG pH 3?0, GE Healthcare, Uppsala, Sweden) was added. After 1 h vortexing at 4uC, samples were centrifuged at 250006g for 30 min at 4uC for supernatants collection. The proteins were precipitated by using the kit PlusOne 2D Cleanup (GE Healthcare, Uppsala, Sweden), as recommended by the manufacturer. The pellets were resuspended in rehydration buffer (8 M urea, 0.5 CHAPS, 10 glycerol, 0.5 IPG buffer pH 3?0, 7 mg/2.5 mL DTT, 0.002 bromophenol blue). Protein concentration was measured in each sample by Bradford protein assay. After quantification, 1000 mg of kidney proteins from each animal of the same group and strain were combined to constitute a pool [16] that was submitted to proteomic analysis in triplicate, as described below.2-DE SeparationRenal proteins (1000 mg) were taken from each pooled sample and mixed in rehydration buffer to a volume of 400 mL which wasProteomic of F Renal Metabolism in Micerequired score of .60. Accuracy between the theoretical and experimental obtained mass and pI were also considered. When 2 or more proteins with high scores were identified in the same spot, they are excluded from analysis. Identified proteins were classified into 6 different categories according to their primary function [18].Statistical AnalysisFor kidney F concentration, the software GraphPad InStat version 4.0 for Windows (GraphPad software Inc., La Jolla, USA) was used. Data were analysed by 2-way ANOVA and Bonferroni test for individual comparisons (p,0.05). For proteomic data, statistical analysis was performed using ANOVA available at ImageMaster 2D Platinum 7.0 soft.He dried gel pieces were rehydrated with 20 mM DTT in 50 mM Ambic for 40 min at 56uC. Excess of reagent was removed and 55 mM iodoacetamide (IAA) in Ambic 50 mM was added for 30 min RT at dark. The remaining liquid was removed and washed out with 25 mM Ambic, followed by dehydration with ACN. After its removal, the gels were dried again. For digestion, dried gels were incubated with 10 ng/mL trypsin in 25 mM Ambic for 15 min (Trypsin Gold Mass spectrometry, Promega, Madison, USA). Peptides were sequentially extracted from the gels initially in 50 ACN (v/v) with 5 formic acid for 14 h at 37uC, then in 50 ACN (v/v) with 1 formic acid for 15 min, followed by 60 methanol (v/v) with 1 formic acid for 15 min and twice with 100 ACN at 45uC under sonication (40kHz/30W, Branson, Danbury, USA). Extracts were dried using a vacuum concentrator (Eppendorf, Hamburg, Germany) and kept at -20uC. Prior to MS identification, dried peptides were dissolved in 12 mL 0.1 formic acid. The peptides were identified 18325633 and quantified by LC-ESI-Q-TOF MS (Liquid Chromatography Electrospray Ionization Quadrupole Time of Flight Mass Spectrometry) (Waters, Mildord, USA). MassLynx 4.1 SCN662 software (Waters, Mildord, USA) was used to submit the combined MS and MS/MS data to MASCOT database search engine (http://www.matrixscience.com) (version 2007.12.04) based on IPI (International Protein Index) protein database restricted to taxonomies Mus musculus (Mouse). The search was limited with a mass tolerance of 100 ppm and only one missed cleavage per peptide was allowed. For modification of peptides, cysteine carbamido-methylation (fixed) and methionine oxidation (variable) were considered. Significant matching proteinSample Preparation for 2DEKidney samples were homogenized using mortar and pestle in liquid nitrogen. Denaturation buffer (7 M urea, 2 M de thioureia, 4 CHAPS, 1 DTT and 0.5 IPG pH 3?0, GE Healthcare, Uppsala, Sweden) was added. After 1 h vortexing at 4uC, samples were centrifuged at 250006g for 30 min at 4uC for supernatants collection. The proteins were precipitated by using the kit PlusOne 2D Cleanup (GE Healthcare, Uppsala, Sweden), as recommended by the manufacturer. The pellets were resuspended in rehydration buffer (8 M urea, 0.5 CHAPS, 10 glycerol, 0.5 IPG buffer pH 3?0, 7 mg/2.5 mL DTT, 0.002 bromophenol blue). Protein concentration was measured in each sample by Bradford protein assay. After quantification, 1000 mg of kidney proteins from each animal of the same group and strain were combined to constitute a pool [16] that was submitted to proteomic analysis in triplicate, as described below.2-DE SeparationRenal proteins (1000 mg) were taken from each pooled sample and mixed in rehydration buffer to a volume of 400 mL which wasProteomic of F Renal Metabolism in Micerequired score of .60. Accuracy between the theoretical and experimental obtained mass and pI were also considered. When 2 or more proteins with high scores were identified in the same spot, they are excluded from analysis. Identified proteins were classified into 6 different categories according to their primary function [18].Statistical AnalysisFor kidney F concentration, the software GraphPad InStat version 4.0 for Windows (GraphPad software Inc., La Jolla, USA) was used. Data were analysed by 2-way ANOVA and Bonferroni test for individual comparisons (p,0.05). For proteomic data, statistical analysis was performed using ANOVA available at ImageMaster 2D Platinum 7.0 soft.