QIAseq Tumor Mutational Burden Panels
For creating a comprehensive profile of Tumor Mutational Burden (TMB) and Microsatellite Instability Status (MSI)
QIAseq Tumor Mutational Burden Panels
For creating a comprehensive profile of Tumor Mutational Burden (TMB) and Microsatellite Instability Status (MSI)
がん研究者は、腫瘍の突然変異の全体の状況を把握するため簡単かつ信頼性のあるワークフローの作成という課題に直面しています。Tumor Mutational Burden(TMB)は、腫瘍内に見出される突然変異数の指標です。しかし標準化された遺伝子検査法がなく、TMBを用いて意義あるバイオマーカーを作製することは困難です。QIAseq Tumor Mutational Burden Panelsは、これまでのアッセイデザインの課題を克服し、全エキソームデータと95%以上の相関を維持しながら、低い偽陰性率で高い解析感度を実現し、TMBとマイクロサテライト不安定性(MSI)の総合プロファイルを作製します。QIAseq TMBおよびMSIパネルを含むQIAseq NGSアッセイは、サンプルのエラー率が5%未満の品質を確保したTMBスコアを提供します。QIAseq TMB Panelsは、いくつかの主要なオピニオンリーダーラボでテストされており、以前の多くの製品と同等以上の性能です。この包括的なパネルは486の遺伝子をカバーし、27のMSIマーカーを追加することが可能です。
Each panel is a one-box, NGS platform-agnostic solution that contains all the necessary components, such as beads and key primers, to construct libraries from enriched genomic targets. Primer design is based on single primer extension, in which each genomic target is enriched by one target-specific primer and one universal primer – a strategy that removes conventional two target-specific primer design restriction and reduces the amount of required primers. All primers required for a panel are pooled into an individual primer pool to reduce panel handling and the number of pools required for enrichment and library construction. Platform-specific indexes, which are contained in a separate box, allow the multiplexing of up to 384 samples per sequencing run.
Performance table QIAseq TMB Panels and MSI:
PCR duplicates are a major issue in targeted DNA sequencing, since, through PCR amplification, they turn unique DNA molecules into identical DNA molecules that cannot be distinguished from each other. In addition, errors from PCR amplification and sequencing process may also be present in final reads that lead to false positive variants in sequencing results. This, in turn, results in the inability to confidently call DNA variants present at low frequencies in the starting DNA material. To overcome the issue of PCR duplicates and amplification artifacts, the QIAseq TMB Panels use digital sequencing by incorporating UMIs into the starting DNA material before any amplification takes place, thereby preserving the uniqueness of the starting DNA molecules and overcoming the issues of PCR duplicates, false positives and library bias.
The entire workflow of the QIAseq TMB Panels to go from extracted DNA to sequencing-ready libraries can be completed in 9 hours (see Figure "Workflow"). Extracted DNA is fragmented, genomic targets are molecularly bar coded and enriched, and libraries are constructed. Sequencing files can be fed into the QIAseq pipeline, a cloud-based data analysis pipeline, which will filter, map and align reads, as well as count unique molecular bar codes associated with targeted genomic regions, and call variants with a bar code-aware algorithm. This data can then be fed into IVA or QCI for interpretation.
The QIAseq TMB Panels can be used to call a variety of DNA variants from a wide range of sample types for numerous applications.
DNA variants:
Sample types:
Applications:
Content: