Відмінності між версіями «SAll experiments involving wild form and transgenic»
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| − | + | SAll experiments involving wild variety and [http://about:blank Al regulation and IBD susceptibilityFig 6. Motif activity response {analysis|evaluation] transgenic mice were reviewed by the IACUC at the Children's Hospital of Philadelphia (protocol no. Mice had been utilized for phenotypic analyses of osteochondroma formation and development in cranial base and other internet sites as in preceding related studies [20, 22, 49]. Handle and compound transgenic mice at P7 or P10 had been provided a single intraperitoneal injection of tamoxifen (1 mg per 13 grs physique weight); stock tamoxifen resolution was 20 mg/ml in ethanol: corn oil mixture at 1:four ratio. When indicated, companions received a equivalent volume of ethanol:corn oil car. Mice had been sacrificed at indicated time points, and body parts and tissues had been processed for imaging along with other procedures as detailed under. For experiments at juvenile stages, we applied Ext1f/f mice [49] mated with Aggrecan-CreERT2 (Agr-CreER) mice [53] to produce compound Agr-CreER;Ext1f/f mice and appropriate controls. Mice at P28 or P35 had been then treated with tamoxifen or vehicle as above. To monitor topography of CreER action, the Agr-CreER mice have been mated with R26-tdTomato reporter mice (Jackson Labs). Compound Agr-CreER;R26-tdTomato mice had been injected with tamoxifen or car at P21, P28 or P35, and limb and craniofacial specimens were harvested two to four days later and processed for histological and fluorescence evaluation of reporter activity as described [78]. Labeling and analysis of proliferative cells by EdU incorporation had been carried out as described [79]. For experiments involving the BMP signaling inhibitor LDN-193189, the drug was dissolved in distilled water at 1 mg/ml stock resolution [58]. Aliquots had been prepared and stored at -80 . Around the day of treatment, an aliquot was thawed and utilized only after to treat mice at 3 mg/kg dose by IP injection when each day to get a total of 6 weeks. Companion controls had been injected with automobile (water). Therapy began one particular day right after tamoxifen injection. Every single group consisted of 3 vehicle-treated and 3 drug-treated mice. We carried out a total of five independent experiments, and data had been made use of to calculate averages and statistical significance.Histological, histochemical, x-ray and CT analysesIndicated body parts and samples were fixed overnight in four paraformaldehyde, washed with 1x PBS for three times and stored in PBS or ethanol at 4 . Complete cranial bases were scanned for CT in coronal and sagittal view utilizing a Viva CT 40 scanner (Scanco Healthcare AG, Switzeland) and analyzed utilizing CT v6.0 vivaCT application as we described previously [80]. Serial 10.5 m 2D and 3D images were acquired at 55 kVp power, 145 A intensity and integration time of 200 msec. Raw CT information have been compiled into 2D gray scale pictures.SAll experiments involving wild variety and transgenic mice have been reviewed by the IACUC in the Children's Hospital of Philadelphia (protocol no. IAC 1400952, principal investigator MP). Animals had been handled, treated and cared for based on the approved protocols and procedures.Transgenic mouse lines, husbandry and drug treatmentLoxP-modified Ext1f/f mice described previously [20] had been mated with Col2a1-CreERT (abbreviated to Col2-CreER) transgenic mice expressing Cre recombinase linked to modified estrogen ligand binding domain under the control of collagen2a1 enhancer sequences [50] to produce compound Col2CreER;Ext1f/f mice. | |
Поточна версія на 01:34, 25 листопада 2017
SAll experiments involving wild variety and Al regulation and IBD susceptibilityFig 6. Motif activity response {analysis|evaluation transgenic mice were reviewed by the IACUC at the Children's Hospital of Philadelphia (protocol no. Mice had been utilized for phenotypic analyses of osteochondroma formation and development in cranial base and other internet sites as in preceding related studies [20, 22, 49]. Handle and compound transgenic mice at P7 or P10 had been provided a single intraperitoneal injection of tamoxifen (1 mg per 13 grs physique weight); stock tamoxifen resolution was 20 mg/ml in ethanol: corn oil mixture at 1:four ratio. When indicated, companions received a equivalent volume of ethanol:corn oil car. Mice had been sacrificed at indicated time points, and body parts and tissues had been processed for imaging along with other procedures as detailed under. For experiments at juvenile stages, we applied Ext1f/f mice [49] mated with Aggrecan-CreERT2 (Agr-CreER) mice [53] to produce compound Agr-CreER;Ext1f/f mice and appropriate controls. Mice at P28 or P35 had been then treated with tamoxifen or vehicle as above. To monitor topography of CreER action, the Agr-CreER mice have been mated with R26-tdTomato reporter mice (Jackson Labs). Compound Agr-CreER;R26-tdTomato mice had been injected with tamoxifen or car at P21, P28 or P35, and limb and craniofacial specimens were harvested two to four days later and processed for histological and fluorescence evaluation of reporter activity as described [78]. Labeling and analysis of proliferative cells by EdU incorporation had been carried out as described [79]. For experiments involving the BMP signaling inhibitor LDN-193189, the drug was dissolved in distilled water at 1 mg/ml stock resolution [58]. Aliquots had been prepared and stored at -80 . Around the day of treatment, an aliquot was thawed and utilized only after to treat mice at 3 mg/kg dose by IP injection when each day to get a total of 6 weeks. Companion controls had been injected with automobile (water). Therapy began one particular day right after tamoxifen injection. Every single group consisted of 3 vehicle-treated and 3 drug-treated mice. We carried out a total of five independent experiments, and data had been made use of to calculate averages and statistical significance.Histological, histochemical, x-ray and CT analysesIndicated body parts and samples were fixed overnight in four paraformaldehyde, washed with 1x PBS for three times and stored in PBS or ethanol at 4 . Complete cranial bases were scanned for CT in coronal and sagittal view utilizing a Viva CT 40 scanner (Scanco Healthcare AG, Switzeland) and analyzed utilizing CT v6.0 vivaCT application as we described previously [80]. Serial 10.5 m 2D and 3D images were acquired at 55 kVp power, 145 A intensity and integration time of 200 msec. Raw CT information have been compiled into 2D gray scale pictures.SAll experiments involving wild variety and transgenic mice have been reviewed by the IACUC in the Children's Hospital of Philadelphia (protocol no. IAC 1400952, principal investigator MP). Animals had been handled, treated and cared for based on the approved protocols and procedures.Transgenic mouse lines, husbandry and drug treatmentLoxP-modified Ext1f/f mice described previously [20] had been mated with Col2a1-CreERT (abbreviated to Col2-CreER) transgenic mice expressing Cre recombinase linked to modified estrogen ligand binding domain under the control of collagen2a1 enhancer sequences [50] to produce compound Col2CreER;Ext1f/f mice.
