SRX1986263
GSM2254825
GSM2254825: A1; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590766
GSM2254825
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254825
GEO Accession
GSM2254825
SRX1986264
GSM2254826
GSM2254826: A2; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590767
GSM2254826
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254826
GEO Accession
GSM2254826
SRX1986265
GSM2254827
GSM2254827: A3; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590768
GSM2254827
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254827
GEO Accession
GSM2254827
SRX1986266
GSM2254828
GSM2254828: A4; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590769
GSM2254828
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254828
GEO Accession
GSM2254828
SRX1986267
GSM2254829
GSM2254829: HK1; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590770
GSM2254829
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254829
GEO Accession
GSM2254829
SRX1986268
GSM2254830
GSM2254830: HK2; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590771
GSM2254830
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254830
GEO Accession
GSM2254830
SRX1986269
GSM2254831
GSM2254831: HK3; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590772
GSM2254831
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254831
GEO Accession
GSM2254831
SRX1986270
GSM2254832
GSM2254832: HK4; Nitrobacter winogradskyi; RNA-Seq
SRP080157
SRS1590773
GSM2254832
RNA-Seq
TRANSCRIPTOMIC
cDNA
Cells were collected by centrifuging, lysed by sonication, and total RNA was extracted with a Qiagen Rneasy Kit. Ribosomal RNA was depleted with a MICROBExpress Bacterial mRNA enrichment kit. An Illumina-targeted RNA Expression Kit and at least 200 ng of RNA containing less than 5% rRNA were used to prepare mRNA-Seq libraries. The libraries were sequenced (150mer paired-end) on a HISEq 3000 Sequencer (Illumina, San Diego, CA) at the Center for Genome Research and Biocomputing Core Laboratories at Oregon State University. mRNA-Seq.
Illumina HiSeq 3000
gds
302254832
GEO Accession
GSM2254832