SNAP-CUTANA™ DYKDDDDK Tag Panel是 CUT&RUN 的加標對照���,提供了一種用于驗證抗 FLAG®* 抗體的分析內對照�����,并證實了涉及FLAG表位標記的染色質蛋白的CUT&RUN反應的成功��。這種重要的陽性對照可指導故障排除�����,以區分 FLAG 表位標記問題(包括轉基因表達�����、標記蛋白的染色質結合、標簽的溶劑可及性等)與 CUT&RUN 工作流程中的技術故障�����。該panel由兩個包含未修飾組蛋白H3或3xDYKDDDDK-H3融合的核小體組成���,每個核小體都包裹有兩個獨-特的條形碼DNA模板(A和B�����,用于內部技術復制)�����。核小體單獨與順磁珠偶聯并匯集到單個panel中��,方便一步加標到CUT&RUN反應�����。在添加抗 DYKDDDDK 或 IgG 陰性對照抗體之前��,將 panel 與 ConA 固定的細胞一起添加(參見應用說明和表 1)�����。pAG-MNase釋放基因組染色質和條形碼核小體取決于所使用抗體的特異性���。測序后���,回收的 DYKDDDDK 與未修飾核小體的相對讀取計數提供了靶向與脫靶回收率的定量指標(圖 2)��,從而衡量實驗成功率并指導故障排除工作��。有關工作流集成���、預期結果、數據分析和故障排除的詳細信息�����,請參閱最新的CUTANA™ CUT&RUN方法(鏈接請聯系Epicypher代理商欣博盛生物獲?��。┖蚐NAP-CUTANA™ Spike-in(鏈接請聯系Epicypher代理商欣博盛生物獲取)用戶指南�����。
*FLAG® is a registered trademark of Merck KGaA, Darmstadt, Germany and ANTI-FLAG is a trademark of Sigma-Aldrich Co. LLC.
保存溫度
自收到之日起��,-20℃下可穩定儲存6個月�����。較低的溫度會導致凍結,并會永-久損壞磁珠�����。
驗證數據
Figure 1: Schematic of SNAP-CUTANA™ DYKDDDDK Tag Panel |
The DYKDDDDK Tag Panel contains two nucleosomes - one has an H3 tail fusion to a 3xDYKDDDDK Tag epitope and one is an unmodified control. Both octamers are wrapped with two uniquely barcoded DNA templates (A and B). Each 250 bp DNA template contains a 123 bp 601 nucleosome positioning sequence (gray) [1], a unique 22 bp DNA-barcode (white; 4 barcodes total), and a 5’ biotin-TEG. The 5’ and 3’ linkers (blue) are compatible with cleavage by pAG-MNase (EpiCypher 14-1048, 15-1016) during CUT&RUN. The nucleosomes are individually pre-conjugated to paramagnetic beads and pooled for convenient use.
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Figure 2: SNAP-CUTANA™ DYKDDDDK Tag Panel provides an in-assay control for CUT&RUN reactions targeting FLAG-tagged proteins |
CUT&RUN was performed as described in Figure 5. CUT&RUN sequencing reads were aligned to the unique DNA barcodes corresponding to each nucleosome in the SNAP-CUTANA™ DYKDDDDK Tag Panel. Data are expressed as a percent relative to on-target recovery (DYKDDDDK Tag set to 100%) or total counts (IgG). IgG antibody results demonstrate equal loading of unmodified and epitope nucleosomes in the panel. DYKDDDDK Tag antibody results show selective enrichment of the DYKDDDDK Tag spike-in nucleosomes, validating all CUT&RUN steps, including DYKDDDDK antibody binding, pAG-MNase cleavage, and wash conditions.
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Table 1: Recommended SNAP-CUTANA™ DYKDDDDK Tag Panel Spike-in dilution for CUT&RUN reactions of varying starting cell number. |
Figure 3: DNA gel data |
Nucleosomes in the SNAP-CUTANA™ DYKDDDDK Tag Panel were resolved via native PAGE and stained with ethidium bromide to confirm intact nucleosome assembly. Lane 1: Free 250 bp DNA used in nucleosome assembly (100 ng). Lane 2: Intact nucleosomes (400 ng).
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Figure 4: Protein gel data |
Coomassie stained SDS-PAGE gel of the nucleosome containing a 3xDYKDDDDK-H3 fusion (1 μg) in the SNAP-CUTANA DYKDDDDK Tag Panel demonstrates the purity of histones in the preparation. Sizes of molecular weight markers and positions of the core histones (H2A, H2B, 3xDYKDDDDK-H3, and H4) are indicated.
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Figure 5: CUT&RUN methods |
CUT&RUN was performed on 500k MDA-MB-231 native cells stably expressing 3xFLAG-tagged GATA3 [1]** using the CUTANA™ ChIC/CUT&RUN Kit v3 (EpiCypher 14-1048). SNAP-CUTANA™ DYKDDDDK Tag Panel was added just prior to the addition of either DYKDDDDK Tag (0.05 μg; EpiCypher 13-2031) or IgG negative control (0.5 μg; EpiCypher 13-0042) antibodies. Library preparation was performed with 5 ng of DNA (or the total amount recovered if less than 5 ng) using the CUTANA™ CUT&RUN Library Prep Kit (EpiCypher 14-1001/14-1002). Libraries were run on an Illumina NextSeq2000 with paired-end sequencing (2x50 bp). Data were aligned to the hg19 genome using Bowtie2. Data were filtered to remove duplicates, multi-aligned reads, and ENCODE DAC Exclusion List regions.
**Thanks to Dr. Takaku (UND) for 3xFLAG-GATA3-3xHA MDA-MB-231 cells. |
訂購詳情
貨號 | 產品名稱 | 規格 |
19-5001 | SNAP-CUTANA™ DYKDDDDK Tag Panel/欣博盛生物 | 50 Reactions |
參考文獻
[1] Lowary & Widom J. Mol. Biol. (1998). PMID: 9514715
[2] Takaku et al. Genome Biol. (2016). PMID: 26922637
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