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Nextera xt dna sample preparation reagents

Manufactured by Illumina
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The Nextera XT DNA Sample Preparation Reagents are a library preparation kit designed for high-throughput sequencing of genomic DNA samples. The kit utilizes a proprietary tagmentation process to simultaneously fragment and tag DNA samples, enabling rapid library construction.

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Lab products found in correlation

Quant it high sensitivity dna assay kit, by Thermo Fisher Scientific (2 mentions) Tcl buffer, by Qiagen (2 mentions) Ampure xp spri beads, by Beckman Coulter (2 mentions) Miseq sequencer, by Illumina (2 mentions) 2 mercaptoethanol, by Merck Group (2 mentions) Smarter ultra low rna kit, by Takara Bio (2 mentions) High sensitivity dna chip, by Agilent Technologies (2 mentions) Nextseq 500, by Illumina (1 mentions)

Spelling variants of this product

Nextera XT (418 citations) Nextera XT DNA (23 citations) Nextera reagents (23 citations) Nextera XT reagents (15 citations)

3 protocols using nextera xt dna sample preparation reagents

1

Single-Cell RNA Sequencing of Circulating Tumor Cells

Cited 1 time
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Single CTCs were recovered, using the nanowell-based isolation platform, into individual wells of a 96 well plate containing 10 µL of buffer TCL (Qiagen) supplemented with 1% 2-mercaptoethanol (Sigma), spun down, snap frozen on dry ice, and stored at −80 °C until further processing. Next, RNA from each single CTC was isolated, reverse transcribed, and amplified using the SMARTer Ultra-low RNA kit (Clontech) as previously described32 (link). Afterwards, cDNA libraries were prepared using Nextera XT DNA Sample preparation reagents (Illumina) as per the manufacturer’s recommendations, with minor modifications. Specifically, reactions were run at ¼ the recommended volume, the tagmentation step was extended to 10 minutes, and the extension time during the PCR step was increased from 30s to 60s. After the PCR step, all 96 samples were pooled without library normalization, cleaned twice with 0.9× AMPure XP SPRI beads (Beckman Coulter), and eluted in Tris-EDTA buffer, pH 8 (Teknova). The pooled libraries were quantified using Quant-IT DNA High-Sensitivity Assay Kit (Invitrogen) and examined using a high sensitivity DNA chip (Agilent). Finally, samples were sequenced using a MiSeq sequencer (Illumina).
Lohr J.G., Adalsteinsson V.A., Cibulskis K., Choudhury A.D., Rosenberg M., Cruz-Gordillo P., Francis J., Zhang C.Z., Shalek A.K., Satija R., Trombetta J.T., Lu D., Tallapragada N., Tahirova N., Kim S., Blumenstiel B., Sougnez C., Lowe A., Wong B., Auclair D., Van Allen E.M., Nakabayashi M., Lis R.T., Lee G.S., Li T., Chabot M.S., Ly A., Taplin M.E., Clancy T.E., Loda M., Regev A., Meyerson M., Hahn W.C., Kantoff P.W., Golub T.R., Getz G., Boehm J.S, & Love J.C. (2014). Whole exome sequencing of circulating tumor cells provides a window into metastatic prostate cancer. Nature biotechnology, 32(5), 479-484.
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2

Single-Cell RNA Sequencing of Circulating Tumor Cells

Cited 1 time
Check if the same lab product or an alternative is used in the 5 most similar protocols
Single CTCs were recovered, using the nanowell-based isolation platform, into individual wells of a 96 well plate containing 10 µL of buffer TCL (Qiagen) supplemented with 1% 2-mercaptoethanol (Sigma), spun down, snap frozen on dry ice, and stored at −80 °C until further processing. Next, RNA from each single CTC was isolated, reverse transcribed, and amplified using the SMARTer Ultra-low RNA kit (Clontech) as previously described32 (link). Afterwards, cDNA libraries were prepared using Nextera XT DNA Sample preparation reagents (Illumina) as per the manufacturer’s recommendations, with minor modifications. Specifically, reactions were run at ¼ the recommended volume, the tagmentation step was extended to 10 minutes, and the extension time during the PCR step was increased from 30s to 60s. After the PCR step, all 96 samples were pooled without library normalization, cleaned twice with 0.9× AMPure XP SPRI beads (Beckman Coulter), and eluted in Tris-EDTA buffer, pH 8 (Teknova). The pooled libraries were quantified using Quant-IT DNA High-Sensitivity Assay Kit (Invitrogen) and examined using a high sensitivity DNA chip (Agilent). Finally, samples were sequenced using a MiSeq sequencer (Illumina).
Lohr J.G., Adalsteinsson V.A., Cibulskis K., Choudhury A.D., Rosenberg M., Cruz-Gordillo P., Francis J., Zhang C.Z., Shalek A.K., Satija R., Trombetta J.T., Lu D., Tallapragada N., Tahirova N., Kim S., Blumenstiel B., Sougnez C., Lowe A., Wong B., Auclair D., Van Allen E.M., Nakabayashi M., Lis R.T., Lee G.S., Li T., Chabot M.S., Ly A., Taplin M.E., Clancy T.E., Loda M., Regev A., Meyerson M., Hahn W.C., Kantoff P.W., Golub T.R., Getz G., Boehm J.S, & Love J.C. (2014). Whole exome sequencing of circulating tumor cells provides a window into metastatic prostate cancer. Nature biotechnology, 32(5), 479-484.
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3

Nextera XT DNA Library Preparation

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WTA products were diluted to a concentration of 0.1 to 0.4 ng/μL, tagmented and amplified using Nextera XT DNA Sample preparation reagents (Illumina, San Diego, CA, USA). Tagmentation was performed according to manufacturer’s instructions, modified to use one-quarter of the recommended volume of reagents, extending tagmentation time to 10 min and extending PCR time to 60s. PCR primers were ordered from Integrated DNA Technologies (Coralville, IA, USA). Nextera products were then cleaned twice using 0.9× SPRIs and eluted in water. The final library was quantified using Qubit and analyzed using a high sensitivity DNA chip. It was then diluted to 2.2 pM and sequenced on a NextSeq 500 (Illumina).
Martin-Gayo E., Cole M.B., Kolb K.E., Ouyang Z., Cronin J., Kazer S.W., Ordovas-Montanes J., Lichterfeld M., Walker B.D., Yosef N., Shalek A.K, & Yu X.G. (2018). A Reproducibility-Based Computational Framework Identifies an Inducible, Enhanced Antiviral State in Dendritic Cells from HIV-1 Elite Controllers. Genome Biology, 19, 10.
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