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xGen™ RNA Library Preparation Kit

Accelerate your RNA-Seq transcriptomics research

The xGen RNA Library Prep Kit offers a fast NGS transcriptomics research workflow. Assemble libraries by either manual or automated workflow directly from 1st strand cDNA synthesis while using your preferred indexing options for the experiment.

xGen NGS—made for RNA library preparation.

Ordering

  • Save time and cost—results in as little as 3.5 hours. Combined with the lower cost, you can process more samples in less time to increase your data output.
  • Supports many workflows with indexing options, automation, and Normalase™ Technology—combinatorial dual indexing up to 96-plex, unique dual indexing up to 1536-plex, and enzymatic library normalization available; automation-friendly.
  • Reliable functionality—maintains ligation efficiency at all supported inputs and no adapter titration required.

Product details

The xGen RNA Library Preparation Kit offers a fast, low-cost transcriptome sequencing workflow for Illumina® platforms. Our RNA library prep kit enables stranded RNA library construction directly from 1st strand cDNA without the requirement for 2nd strand cDNA synthesis and degradation, or template-switching methods. This easily automatable kit is compatible with upstream and downstream enrichment and depletion methods and supports a variety of indexing options. These include upstream mRNA enrichment and rRNA depletion modules as well as downstream xGen Hybridization capture workflows for targeted RNA sequencing.

Table 1. Research applications 

Application xGen RNA Library Prep Kit
Gene expression profiling
Research on disease-associated transcripts
Total RNA + hybridization capture enrichment

Automation

The xGen RNA Library Prep Kit protocol is readily automatable. A 10% overage volume of reagents is supplied to accommodate automation, and additional reagent overage volume is available upon request. 

Table 2. Product specifications

Feature Specification Benefit
Input quantity 100 ng to 1 μg total RNA
5 ng to 100 ng mRNA 		Supports a wide input range
RNA types supported Poly(A)-enriched mRNA
Ribo-depleted RNA
Total RNA 		Supports most RNA applications
Technology Adaptase tailing and ligation to 1st strand cDNA Maintains strandedness (≥97%)
No 2nd strand cDNA
No adapter titration
Workflow time* 3.5 hours Less hands-on time
Kit reaction sizes 16, 96, and 4x96 Evaluation and adoption
Components provided Fragmentation module
RT module
Library prep
Polymerase 		Complete solution for processing total, enriched, or depleted RNA from transcript to library
Indexing options Combinatorial dual
Unique dual
Normalase 		Flexible to sequencers, workflows, and applications
Multiplexing capability Up to 1536 libraries Save sequencing costs
Automation Compatible with liquid handlers
Custom packaging available 		Adopt at scale

*Workflow time is based upon incubation times and expected times for hands-on-steps. Actual workflow time may vary depending on individual factors in your laboratory.

Workflow

Reverse transcription—During this step, RNA fragmentation, reverse transcription, and incorporation of the R1 Stubby Adapter are performed, followed by a purification step. 

Adaptase technology—This step performs 3’ tailing and ligation of the R2 Stubby Adapter to first strand cDNA

Indexing PCR—This step completes adapter sequences, adds sample-specific index sequences, and increases library yield, followed by a purification step.

Figure 1. xGen RNA Library Prep Kit workflow converts RNA directly into an indexed library. The workflow for creating an RNA-seq library using the xGen RNA Library Prep Kit includes a proprietary Adaptase technology step that adds a single-stranded R2 Stubby Adapter onto the 3’ end of the 1st strand cDNA product. Indexing primers are then used to amplify the library and add the full-length adapter sequence. See text for details.

Index and kit options

The xGen RNA Library Prep Kit uses primers that anneal to the Stubby Adapters added during the random priming and Adaptase steps, to be fully compatible with Illumina® sequencers. IDT supplies a variety of index configurations and strategies, including:

  • Combinatorial dual indexing, up to 96 combinations
  • Unique dual indexing, up to 1536 unique dual indices

Product data

Save time with direct conversion of 1st strand cDNA

Incubation times for enzymatic and purification steps are shown according to vendor supplied user instructions.

Figure 2. Comparison of different workflow times for RNA-seq library preparation kits. The xGen RNA Library Prep Kit constructs library molecules directly from 1st strand cDNA synthesis, which reduces the time from fragmentation (F) to clean-up (C).

Reliable mapping and strandedness

The xGen RNA Library Kit shows high mapping rates and maintenance of strandedness.

Figure 3. Reliable mapping rate and strandedness with the xGen RNA Library Prep Kit. (A) Universal Human Reference (UHR) Total RNA (Agilent) was enriched using the NEBNext Poly(A) mRNA Magnetic Isolation Module (NEB). Libraries were constructed from 50, 100, and 250 ng of enriched mRNA using the xGen RNA Library Prep Kit and the Supplier K’s kit according to the manufacturer’s instructions. (B) Human Brain mRNA (Clontech) was used to construct the xGen RNA and the Supplier K’s libraries from 1, 5, 10, 50, 100 ng of Human mRNA. The percent strandedness was determined by the average of the five input quantities. For both graph A and graph B, libraries were sequenced on a MiniSeqTM with 2 X 75 bp paired-end reads. Fastq files were downsampled to 3.8 million reads before analysis using STAR (mapping rate) or RNA-SeQC (strandedness).

Frequently asked questions

The Swift products were rebranded and now belong to the xGen™ NGS product line. The following lists the old Swift product name, and then the new name hyperlinked to its current product page.

Swift product name New IDT product name
Accel-NGS® Adaptase® Module for Single-Cell Methyl-Seq xGen Adaptase™ Module
Normalase® Amplicon Panels (SNAP) Core xGen Amplicon Core
SARS-CoV-2 Additional Genome Coverage Panel xGen SARS-CoV-2 Expanded Amplicon Panel
SARS-CoV-2 S Gene Panel xGen SARS-CoV-2 SGene Amplicon Panel
SNAP Set 1A Combinatorial Dual Indexing Primers xGen Amplicon CDI Primers
Swift Combinatorial Dual Indexing Primers xGen CDI Primers
Swift Normalase® Combinatorial Dual Indexing Primers xGen Normalase CDI Primers
Accel-NGS 1S Plus DNA Library xGen ssDNA & Low-input DNA Library Prep
Swift 2S Sonic DNA Library xGen DNA Library Prep MC
Swift 2S Sonic Flexible DNA Library xGen DNA Library Prep MC UNI
Swift 2S Turbo v2 xGen DNA Library Prep EZ
Swift 2S Turbo Flexible v2 DNA Library xGen DNA Library Prep EZ UNI
Accel-NGS Methyl-Seq DNA Library xGen Methyl-Seq Library Prep
Swift Normalase xGen Normalase Module
Swift Rapid RNA Library xGen RNA Library Prep Kit
Swift RNA Library xGen Broad-Range RNA Library Prep

View FAQ

No, this kit takes as input one of the following:

1. Total RNA

2. mRNA that has already been enriched by poly(A) selection

3. RNA that has already been depleted of rRNA

The xGen RNA Library Prep Kit begins with an RNA fragmentation and reverse transcription step. Therefore, if mRNA enrichment or ribodepletion is desired, one of the kits below is required and recommended for pre-processing. These kits have been tested for compatibility with the xGen RNA Library Prep Kit.

Note: View this xGen RNA Library Prep Kit Protocol for instructions on matching the output of these upstream modules with the initial steps of the xGen RNA Library Prep Kit.

Method Recommended kit Alternate kit
Poly(A) mRNA enrichment NEBNext® Poly (A) mRNA Magnetic Isolation Module
Cat. No. E7490
Lexogen Poly (A) RNA Selection Kit
Cat. No. 039.100
Ribodepletion Lexogen RiboCop rRNA Depletion Kit V1.2 (Human/Mouse/Rat)
Cat. No. 037.24/96
NEBNext rRNA Depletion Kit (Human/Mouse/Rat)
Cat. No. E6310S/L/X

View FAQ

The xGen™ RNA Library Prep Kits have an Indexing PCR step to complete the fully indexed adapter sequences following ligation of stubby adapters during the library prep workflows so they are fully compatible with Illumina® sequencers.

IDT supplies a variety of index configurations and strategies, including dual indexing as either:

  • Combinatorial dual indexing, up to 96 combinations
  • Unique dual indexing, up to 1536 combinations

View FAQ

The xGen™ RNA Library Prep Kit uses three main steps:

  1. Fragmentation & Reverse Transcription, where RNA is fragmented and converted to cDNA. Because the random primer is tailed, the 1st strand cDNA already contains the Read 1 Stubby Adapter.
  2. Adaptase, where the Read 2 Stubby Adapter is added to the 3’ end of 1st strand cDNA.
  3. Indexing PCR, where simultaneously the fully indexed adapter sequences are added, and the library is amplified to generate sufficient yield for sequencing.

View FAQ

The shelf life of the xGen RNA Library Prep Kit is at least 6 months from the time the product is delivered when stored as required at –20°C and handled according to the protocol.

The enzymes provided in this kit are temperature sensitive, and appropriate care should be taken during handling and storage. Upon receipt, store the kits at –20°C.

View FAQ

We obtained sequencing results with the xGen RNA Library Prep Kit Protocol using inputs from 100 ng to 1 µg of total RNA into an upstream module, 5–100 ng of mRNA into library prep, or up to 500 ng of total RNA into library prep for downstream hybridization capture.

View FAQ

Accurate library quantification is essential to properly load the sequencing instrument. Libraries can be quantified using fluorometric-, electrophoretic-, or qPCR-based methods. Electrophoresis-based methods also help with the examination of library insert size distribution. There are many commercially available kits suitable for library quantification. 

Following the recommended PCR cycles in the xGen RNA Library Prep Kit Protocol will result in a library concentration of at least 4 nM. 

The  xGen™ RNA Library Prep Kit can also be used with the Normalase™ Module to generate 2 nM or 4 nM normalized library pools.
 

View FAQ

No.

The xGen™ RNA Library Prep Kit does not require adapter titration at any of the supported input levels. Adapter ligation efficiency is maintained at all supported input quantities.

View FAQ

Go to Appendix H: Indexed adapter sequences in the xGen RNA Library Prep Kit Protocol for details about the adapter sequences and structure of the xGen™ RNA Library Prep Kit adapters and indexing primer kits.

Please contact Scientific Application Support at applicationsupport@idtdna.com if you wish to confirm compatibility of your own custom indexing primers with the stubby adapters supplied in the xGen RNA Library Prep Kit workflows.

View FAQ

Adaptase™ technology, used in the xGen™ RNA Library Prep Kit, adds a low complexity polynucleotide tail with a median length of eight bases to the 3’ end of each fragment during the addition of the second NGS adapter molecule (Read 2 Stubby Adapter). Considering this, it is normal and expected to observe them at the beginning of Read 2 (R2).

When read length is close to fragment size, the tail may also be observed toward the end of Read 1 (R1). We recommend using the STAR aligner (Dobin et al. 2013) as it can soft clip the synthetic tail sequence and provides efficient mapping without additional processing of your sequencing data.

For more details, refer to Appendix G: Data analysis and informatics in the xGen RNA Library Prep Kit Protocol.

View FAQ

Yes.

The Indexing PCR step is a required step to complete the indexed adapter sequences and generate sufficient library for sequencing.

Refer to the xGen RNA Library Prep Kit Protocol for specific cycle requirements based on input RNA quantity.

View FAQ

Yes.

Refer to the Appendix section of the xGen RNA Library Prep Kit Protocol titled 'Expected Results with Alternate Fragmentation Times'.

Appendix F provides details on fragmentation times and bead cleanup ratios required for different intended mean library sizes ranging from 380–480 bp (mean insert sizes ranging from 250–350 bp).

 

View FAQ

The xGen™ RNA Library Prep Kit includes a stubby adapter in the workflow so the stocked UDI-UMI adapters are not compatible with those kits.

For customers using homebrew, or other commercial RNA-seq workflows that utilize TA-ligation, these UDI-UMI adapters are compatible. However, it is important to note that stranded RNA-seq libraries constructed using xGen UDI-UMI Adapters have the insert strandedness flipped (i.e., to the opposite strand) when compared to standard Illumina TruSeq™ adapters. As such, this strand flip must be handled during data analysis.

Disclaimer: TruSeq™ and Nextera™ are registered trademarks of Illumina, Inc., used with permission. All rights reserved.

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