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EpiCypher新品介紹:SNAP-CUTANA™ DYKDDDDK Tag Panel

更新時(shí)間:2024-03-13   點(diǎn)擊次數(shù):366次

SNAP-CUTANA™ DYKDDDDK Tag Panel是 CUT&RUN 的加標(biāo)對(duì)照,提供了一種用于驗(yàn)證抗 FLAG®* 抗體的分析內(nèi)對(duì)照,并證實(shí)了涉及FLAG表位標(biāo)記的染色質(zhì)蛋白的CUT&RUN反應(yīng)的成功。這種重要的陽(yáng)性對(duì)照可指導(dǎo)故障排除,以區(qū)分 FLAG 表位標(biāo)記問(wèn)題(包括轉(zhuǎn)基因表達(dá)、標(biāo)記蛋白的染色質(zhì)結(jié)合、標(biāo)簽的溶劑可及性等)與 CUT&RUN 工作流程中的技術(shù)故障。該panel由兩個(gè)包含未修飾組蛋白H3或3xDYKDDDDK-H3融合的核小體組成,每個(gè)核小體都包裹有兩個(gè)獨(dú)-特的條形碼DNA模板(A和B,用于內(nèi)部技術(shù)復(fù)制)。核小體單獨(dú)與順磁珠偶聯(lián)并匯集到單個(gè)panel中,方便一步加標(biāo)到CUT&RUN反應(yīng)。在添加抗 DYKDDDDK 或 IgG 陰性對(duì)照抗體之前,將 panel 與 ConA 固定的細(xì)胞一起添加(參見應(yīng)用說(shuō)明和表 1)。pAG-MNase釋放基因組染色質(zhì)和條形碼核小體取決于所使用抗體的特異性。測(cè)序后,回收的 DYKDDDDK 與未修飾核小體的相對(duì)讀取計(jì)數(shù)提供了靶向與脫靶回收率的定量指標(biāo)(圖 2),從而衡量實(shí)驗(yàn)成功率并指導(dǎo)故障排除工作。有關(guān)工作流集成、預(yù)期結(jié)果、數(shù)據(jù)分析和故障排除的詳細(xì)信息,請(qǐng)參閱最新的CUTANA™ CUT&RUN方法(鏈接請(qǐng)聯(lián)系Epicypher代理商欣博盛生物獲?。┖蚐NAP-CUTANA™ Spike-in(鏈接請(qǐng)聯(lián)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(wěn)定儲(chǔ)存6個(gè)月。較低的溫度會(huì)導(dǎo)致凍結(jié),并會(huì)永-久損壞磁珠。


驗(yàn)證數(shù)據(jù)

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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 14-104815-1016) during CUT&RUN. The nucleosomes are individually pre-conjugated to paramagnetic beads and pooled for convenient use.

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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.

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

Table 1: Recommended SNAP-CUTANA™ DYKDDDDK Tag Panel Spike-in dilution for CUT&RUN reactions of varying starting cell number.

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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).

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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.

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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(gòu)詳情

貨號(hào)

產(chǎn)品名稱

規(guī)格

19-5001

SNAP-CUTANA™ DYKDDDDK Tag Panel/欣博盛生物

50 Reactions


參考文獻(xiàn)

[1] Lowary & Widom J. Mol. Biol. (1998). PMID: 9514715

[2] Takaku et al. Genome Biol. (2016). PMID: 26922637


 

EpiCypher新品推薦——SNAP-CUTANA™ DYKDDDDK Tag Panel

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