SRX7115118 GSM4154220 SRP229091 SRS5625891 GSM4154220 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154220 GSM4154220 GEO Accession GSM4154220 SRX7115119 GSM4154221 SRP229091 SRS5625892 GSM4154221 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154221 GSM4154221 GEO Accession GSM4154221 SRX7115120 GSM4154222 SRP229091 SRS5625893 GSM4154222 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154222 GSM4154222 GEO Accession GSM4154222 SRX7115121 GSM4154223 SRP229091 SRS5625894 GSM4154223 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154223 GSM4154223 GEO Accession GSM4154223 SRX7115122 GSM4154224 SRP229091 SRS5625895 GSM4154224 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154224 GSM4154224 GEO Accession GSM4154224 SRX7115123 GSM4154225 SRP229091 SRS5625896 GSM4154225 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154225 GSM4154225 GEO Accession GSM4154225 SRX7115124 GSM4154226 SRP229091 SRS5625897 GSM4154226 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154226 GSM4154226 GEO Accession GSM4154226 SRX7115125 GSM4154227 SRP229091 SRS5625898 GSM4154227 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154227 GSM4154227 GEO Accession GSM4154227 SRX7115126 GSM4154228 SRP229091 SRS5625899 GSM4154228 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154228 GSM4154228 GEO Accession GSM4154228 SRX7115127 GSM4154229 SRP229091 SRS5625900 GSM4154229 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154229 GSM4154229 GEO Accession GSM4154229 SRX7115128 GSM4154230 SRP229091 SRS5625901 GSM4154230 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154230 GSM4154230 GEO Accession GSM4154230 SRX7115129 GSM4154231 SRP229091 SRS5625902 GSM4154231 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154231 GSM4154231 GEO Accession GSM4154231 SRX7115130 GSM4154232 SRP229091 SRS5625903 GSM4154232 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154232 GSM4154232 GEO Accession GSM4154232 SRX7115131 GSM4154233 SRP229091 SRS5625904 GSM4154233 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154233 GSM4154233 GEO Accession GSM4154233 SRX7115132 GSM4154234 SRP229091 SRS5625905 GSM4154234 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154234 GSM4154234 GEO Accession GSM4154234 SRX7115133 GSM4154235 SRP229091 SRS5625906 GSM4154235 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154235 GSM4154235 GEO Accession GSM4154235 SRX7115134 GSM4154236 SRP229091 SRS5625907 GSM4154236 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154236 GSM4154236 GEO Accession GSM4154236 SRX7115135 GSM4154237 SRP229091 SRS5625908 GSM4154237 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154237 GSM4154237 GEO Accession GSM4154237 SRX7115136 GSM4154238 SRP229091 SRS5625909 GSM4154238 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154238 GSM4154238 GEO Accession GSM4154238 SRX7115137 GSM4154239 SRP229091 SRS5625910 GSM4154239 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154239 GSM4154239 GEO Accession GSM4154239 SRX7115138 GSM4154240 SRP229091 SRS5625911 GSM4154240 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154240 GSM4154240 GEO Accession GSM4154240 SRX7115139 GSM4154241 SRP229091 SRS5625912 GSM4154241 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154241 GSM4154241 GEO Accession GSM4154241 SRX7115140 GSM4154242 SRP229091 SRS5625913 GSM4154242 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154242 GSM4154242 GEO Accession GSM4154242 SRX7115141 GSM4154243 SRP229091 SRS5625914 GSM4154243 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154243 GSM4154243 GEO Accession GSM4154243 SRX7115142 GSM4154244 SRP229091 SRS5625915 GSM4154244 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154244 GSM4154244 GEO Accession GSM4154244 SRX7115143 GSM4154245 SRP229091 SRS5625916 GSM4154245 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154245 GSM4154245 GEO Accession GSM4154245 SRX7115144 GSM4154246 SRP229091 SRS5625917 GSM4154246 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154246 GSM4154246 GEO Accession GSM4154246 SRX7115145 GSM4154247 SRP229091 SRS5625918 GSM4154247 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154247 GSM4154247 GEO Accession GSM4154247 SRX7115146 GSM4154248 SRP229091 SRS5625919 GSM4154248 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154248 GSM4154248 GEO Accession GSM4154248 SRX7115147 GSM4154249 SRP229091 SRS5625920 GSM4154249 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154249 GSM4154249 GEO Accession GSM4154249 SRX7115148 GSM4154250 SRP229091 SRS5625921 GSM4154250 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154250 GSM4154250 GEO Accession GSM4154250 SRX7115149 GSM4154251 SRP229091 SRS5625922 GSM4154251 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154251 GSM4154251 GEO Accession GSM4154251 SRX7115150 GSM4154252 SRP229091 SRS5625923 GSM4154252 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154252 GSM4154252 GEO Accession GSM4154252 SRX7115151 GSM4154253 SRP229091 SRS5625924 GSM4154253 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154253 GSM4154253 GEO Accession GSM4154253 SRX7115152 GSM4154254 SRP229091 SRS5625925 GSM4154254 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154254 GSM4154254 GEO Accession GSM4154254 SRX7115153 GSM4154255 SRP229091 SRS5625926 GSM4154255 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154255 GSM4154255 GEO Accession GSM4154255 SRX7115154 GSM4154256 SRP229091 SRS5625927 GSM4154256 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154256 GSM4154256 GEO Accession GSM4154256 SRX7115155 GSM4154257 SRP229091 SRS5625928 GSM4154257 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154257 GSM4154257 GEO Accession GSM4154257 SRX7115156 GSM4154258 SRP229091 SRS5625929 GSM4154258 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154258 GSM4154258 GEO Accession GSM4154258 SRX7115157 GSM4154259 SRP229091 SRS5625930 GSM4154259 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154259 GSM4154259 GEO Accession GSM4154259 SRX7115158 GSM4154260 SRP229091 SRS5625931 GSM4154260 RNA-Seq TRANSCRIPTOMIC cDNA Skeletal muscle samples were homogenized in a Bead Ruptor Elite bead mill homogenizer cooled by liquid nitrogen to 10°C for 2 x 20 seconds at 4.2 m/s. Muscle homogenates were processed using the Agencourt RNAdvance Tissue Kit on a BioMek FXP Laboratory Automation Workstation cDNA libraries were constructed from 250 ng of total RNA using the Universal Plus mRNA-Seq kit from NuGEN Illumina NovaSeq 6000 gds 304154260 GSM4154260 GEO Accession GSM4154260