Click-iT™ TUNEL Alexa Fluor Imaging Assays for Microscopy & HCS
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Invitrogen™

Click-iT™ TUNEL Alexa Fluor Imaging Assays for Microscopy & HCS

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Click-iT TUNELアッセイキットにより、アポトーシス細胞のスクリーニングが可能であり、Alexa Fluor色素を簡単に取り込んでGFPおよびRFPでマルチプレックス化できます。
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製品番号(カタログ番号)標識または色素
C10247遠赤色Alexa Fluor™ 647、Hoechst 33342
C10246RedAlexa Fluor™ 594、Hoechst 33342
C10245GreenAlexa Fluor™ 488、Hoechst 33342
製品番号(カタログ番号) C10247
価格(JPY)
175,500
Each
お問い合わせください ›
色:
遠赤色
標識または色素:
Alexa Fluor™ 647、Hoechst 33342
Click-iT TUNEL Alexa Fluor 488、594、および647イメージングアッセイを使用すると、アポトーシス細胞をわずか2時間で簡単かつ効率的にスクリーニングできます。これらのTUNELアッセイキットは、顕微鏡およびハイコンテントスクリーニング(HCS)での使用を目的としており、銅触媒反応によって断片化DNAのDNA末端に組み込まれたアルキン修飾dUTPを検出します。他の修飾ヌクレオチドを使用するアッセイと比較すると、これらのアポトーシス検出キットは、同一条件下で迅速に(2時間以内に完了)、より高率にアポトーシス細胞を検出できます。Click-iT TUNELアッセイでは、GFPまたはRFPからの蛍光シグナルを測定する方法など、表面および細胞内バイオマーカー検出法による多重化も可能です。
アポトーシスは、細胞の丸み、ブレブ形成、DNA断片化などの明確な細胞過程によって特徴付けられます。TUNELアッセイは、組織サンプルでアポトーシス細胞中の断片化DNAを検出するためにもっとも汎用されている方法です。この場合、まず断片化されたDNAの3’-OH末端に修飾dUTPを取り込みます。dUTPは多くの場合、蛍光色素分子を含んでいます。蛍光色素分子サイズのために、修飾dUTPは予想される取り込み速度よりも低く表示され、TUNELアッセイの感度に悪影響をおよぼす可能性があります。現在市販されているTUNELアッセイキット向け蛍光色素には、光退色や蛍光スペクトルのオーバーラップの問題が多く見られ、いずれもアッセイの感度と多重化能力を低下させます。

Click-iT Plus TUNELアッセイは、これらの問題に対処するために開発されたもので、アジドとアルキルインの間の銅(I)触媒(クリック)反応に基づいています。大型(MW約100,000 Da)抗体と比較した場合、分子量が約1 kDaのAlexa Fluorアジドの小型サイズであるため、Alexa Fluor 488、594、または647色素を複雑なサンプルに簡単に組み込むことができます。これにより、穏やかな固定または透過化が可能になり、アッセイの所要時間が短縮されるため(約2時間)、同一条件下でより高い割合のアポトーシス細胞を検出できます。Click-iT Plus TUNELアッセイは、反応条件が穏やかなため、蛍光タンパク質または色素によるマルチプレックス化が可能です。

Click-iT TUNEL Alexa Fluorイメージングアッセイには、カバースリップまたは96ウェルマイクロプレート上で培養された接着細胞のアポトーシスを正確かつ確実に検出するためのコンポーネントがすべて含まれています。ポジティブコントロール用にストランドブレークを生成するDNase Iも含まれます。
For Research Use Only. Not for use in diagnostic procedures.
仕様
遠赤色
概要Click-iT TUNEL Alexa Fluor™ 647 Imaging Assay
励起/発光650/665
使用対象 (装置)蛍光顕微鏡、ハイコンテント機器
標識タイプAlexa Fluor™色素、クラシック色素
標識または色素Alexa Fluor™ 647、Hoechst 33342
反応数96回の試験または50個のカバースリップ x 1
製品ラインClick-iT
製品タイプImaging Assay
数量1 kit
出荷条件ドライアイス
保存要件遮光し、≤-20℃で保存。
検出法蛍光
フォーマット96ウェルプレート
Unit SizeEach

よくあるご質問(FAQ)

固定・透過処理したサンプルでアポトーシスの確認をしたい。 どの試薬がおすすめか? 蛍光標識 Annexin V は使用できるか?

固定後のサンプルでの Annexin V の使用はお勧めできません。 ホルムアルデヒドによる架橋により、ホスファチジルセリンもマスクされる可能性があるためです。 固定後のサンプルで使用できるアポトーシス検出方法は、anti-Caspase抗体を用いた免疫染色、もしくは、 Click-iT® TUNEL Imaging Kit などの TUNEL法です。

I need to test cells for apoptosis after they have been formaldehyde-fixed and permeabilized. What dye or conjugate do you recommend? Will Annexin V conjugates work?

We do not recommend Annexin V for post-fix labeling, since fixation inactivates the function of the translocase; fixed samples would show mostly uniform labeling with Annexin V. The only options you have for apoptosis assays after fixation are to use an anti-caspase antibody or perform a TUNEL assay, such as with the Click-iT TUNEL Imaging kits.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

Can I use Click-iT TUNEL Alexa Fluor Imaging Assays for Microscopy & HCS (Cat. No. C10246) for flow cytometry?

We have not validated the use of Click‐iT TUNEL assay for flow cytometry. Theoretically, any Click‐iT TUNEL assay for imaging can be adapted to be used with flow cytometry. In general, follow the protocol as provided but spin down the suspension cells after every step. Start with about 10∧6 cells at about 10∧7 cell/mL. Please note that flow cytometry is more sensitive than fluorescence imaging, so you should use between 1/5th to 1/10th of the azide dye detection reagent in the click reaction. All other concentrations of the click reaction reagents should stay the same. We recommend using the Click‐iT Plus TUNEL assays (C10617, C10618, C10619), as the detection reagent is provided in a separate vial, enabling you to modify the concentration used. The Click‐iT Plus TUNEL assay protocol can be found on the following link.

Find additional tips, troubleshooting help, and resources within our Cell Viability, Proliferation, Cryopreservation, and Apoptosis Support Center.

I am observing no signal or very low specific signal for my click-labeled samples. What can I do to improve the signal?

The click reaction is only effective when copper is in the appropriate valency. Azides and alkynes will not react with each other without copper. Make sure that the click reaction mixture is used immediately after preparation when the copper (II) concentration is at its highest.
Do not use additive buffer that has turned yellow; it must be colorless to be active.
Cells need to be adequately fixed and permeabilized for the TdT enzyme and click reagents to have access to the nucleus. Tissue samples require digestion with proteinase K or other proteolytic enzymes for sufficient TdT access.
Some reagents can bind copper and reduce its effective concentration available to catalyze the click reaction. Do not include any metal chelator (e.g., EDTA, EGTA, citrate, etc.) in any buffer or reagent prior to the click reaction. Avoid buffers or reagents that include other metal ions that may be o xidized or reduced. It may be help to include extra wash steps on the cell or tissue sample before performing the click reaction.
You can repeat the click reaction with fresh reagents to try to improve signal. Increasing the click reaction time longer than 30 minutes will not improve a low signal. Performing a second, 30 minute incubation with fresh click reaction reagents is more effective at improving labeling.
Your cells may not be apoptotic. Prepare a DNase I-treated positive control to verify that the TdT enzymatic reaction and click labeling reaction are working correctly.

Find additional tips, troubleshooting help, and resources within our Labeling Chemistry Support Center.

I am observing high non-specific background when I image my Click-iT EdU TUNEL-labeled samples. What is causing this and what can I do to reduce the background?

The click reaction is very selective between an azide and alkyne. No other side reactions are possible in a biological system. Any non-specific background is due to non-covalent binding of the dye to various cellular components. The Select FX Signal Enhancer is not effective at reducing non-specific charge-based binding of dyes following the click reaction; we do not recommend its use with the Click-iT detection reagents. The best method to reduce background is to increase the number of BSA washes. You should always do a no-dye or no-click reaction control under the same processing and detection conditions to verify that the background is actually due to the dye and not autofluorescence. You should also perform the complete click reaction on a no-TdT enzyme control sample to verify the specificity of the click reaction signal.

Find additional tips, troubleshooting help, and resources within our Cell Analysis Support Center.

View all Click-iT™ TUNEL Alexa Fluor Imaging Assays for Microscopy & HCS FAQs

引用および参考文献 (30)

引用および参考文献
Abstract
Auxin-induced Rapid Degradation of Inhibitor of Caspase-activated DNase (ICAD) Induces Apoptotic DNA Fragmentation, Caspase Activation, and Cell Death: A CELL SUICIDE MODULE.
Authors:Samejima K, Ogawa H, Ageichik AV, Peterson KL, Kaufmann SH, Kanemaki MT, Earnshaw WC,
Journal:
PubMed ID:25248749
'Caspase-activated DNase (CAD) is a major apoptotic nuclease, responsible for DNA fragmentation and chromatin condensation during apoptosis. CAD is normally activated in apoptosis as a result of caspase cleavage of its inhibitory chaperone ICAD. Other aspects of CAD regulation are poorly understood. In particular, it has been unclear whether direct ... More
Oxidative and endoplasmic reticulum stresses mediate apoptosis induced by modified LDL in human retinal Müller cells.
Authors:Wu M, Yang S, Elliott MH, Fu D, Wilson K, Zhang J, Du M, Chen J, Lyons T,
Journal:Invest Ophthalmol Vis Sci
PubMed ID:22678501
'We previously showed that extravasated, modified LDL is implicated in pericyte loss in diabetic retinopathy (DR). Here, we investigate whether modified LDL induces apoptosis in retinal Müller glial cells. Cultured human retinal Müller cells (MIO-M1) were treated with highly oxidized glycated LDL (HOG-LDL, 200 mg protein/L) or native LDL (N-LDL, ... More
Varicella-zoster virus infection of differentiated human neural stem cells.
Authors:Pugazhenthi S, Nair S, Velmurugan K, Liang Q, Mahalingam R, Cohrs RJ, Nagel MA, Gilden D,
Journal:J Virol
PubMed ID:21525352
'Primary varicella-zoster virus (VZV) infection in humans produces varicella (chickenpox), after which the virus becomes latent in ganglionic neurons. Analysis of the physical state of viral nucleic acid and virus gene expression during latency requires postmortem acquisition of fresh human ganglia. To provide an additional way to study the VZV-host ... More
Expression of a naturally occurring angiotensin AT(1) receptor cleavage fragment elicits caspase-activation and apoptosis.
Authors:Cook JL, Singh A, DeHaro D, Alam J, Re RN,
Journal:Am J Physiol Cell Physiol
PubMed ID:21813711
'Several transmembrane receptors are documented to accumulate in nuclei, some as holoreceptors and others as cleaved receptor products. Our prior studies indicate that a population of the 7-transmembrane angiotensin type-1 receptor (AT(1)R) is cleaved in a ligand-augmented manner after which the cytoplasmic, carboxy-terminal cleavage fragment (CF) traffics to the nucleus. ... More
Astrocytes secrete exosomes enriched with proapoptotic ceramide and prostate apoptosis response 4 (PAR-4): potential mechanism of apoptosis induction in Alzheimer disease (AD).
Authors:Wang G, Dinkins M, He Q, Zhu G, Poirier C, Campbell A, Mayer-Proschel M, Bieberich E,
Journal:J Biol Chem
PubMed ID:22532571
'Amyloid protein is well known to induce neuronal cell death, whereas only little is known about its effect on astrocytes. We found that amyloid peptides activated caspase 3 and induced apoptosis in primary cultured astrocytes, which was prevented by caspase 3 inhibition. Apoptosis was also prevented by shRNA-mediated down-regulation of ... More
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