Annexin V Conjugates for Apoptosis Detection

Citations & References (14)

Invitrogen™

Annexin V Conjugates for Apoptosis Detection

Name: Annexin V Conjugates for Apoptosis Detection
SKU: A13203

アネキシンVスタンドアロンAlexa Fluor、APC、Pacific Blue、PE、FITC、およびフローサイトメトリーを使用したビオチンコンジュゲートでアポトーシスの初期段階を検出します。

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製品番号（カタログ番号）	励起／発光	フローサイトメーターレーザーライン	コンジュゲート
A13203	590／617	532	Alexa Fluor 594
A13201	495／519	488	Alexa Fluor 488
A13199	494／518	488	FITC
A13202	578／603	532、561	Alexa Fluor 568
A13204			ビオチン-X
A23202	346／442	UV	Alexa Fluor 350
A23204	650／665	633～637	Alexa Fluor 647
A35108	555／565	532、561	Alexa Fluor 555
A35109	679／702	633～637	Alexa Fluor 680
A35110	650/660	633～637	APC（アロフィコシアニン）
A35111	565/578	488、532、561	PE
A35122	410／455	405	Pacific Blue

12 オプション

製品番号（カタログ番号） A13203

価格（JPY）

112,600

Each

お問い合わせください ›

励起／発光:

590／617

フローサイトメーターレーザーライン:

532

コンジュゲート:

Alexa Fluor 594

アポトーシス検出用のアネキシンVスタンドアロンコンジュゲートにより、初期の細胞アポトーシスを迅速かつ信頼性の高い方法で検出できます。アネキシンVコンジュゲートは、フローサイトメトリーを用いたアポトーシス細胞と非アポトーシス細胞の蛍光シグナル強度の差を最大100倍にします。

アネキシンVはホスファチジルセリン（PS）に対する高い親和性を有しており、アポトーシスを受けている細胞の外側のリーフレットに曝露されます。この親和性により、蛍光標識アネキシンV試薬はアポトーシス研究で一般的に使用されます。

アネキシンVコンジュゲートは、アポトーシスの中間期指標であるホスファチジルセリンの外在化を研究するための迅速で信頼性の高い検出法を提供します。フローサイトメトリーで測定した当社の蛍光アネキシンVコンジュゲートで染色したアポトーシス細胞と非アポトーシス細胞の蛍光強度の差は、通常約100倍です。

Nexins Research社との提携により、当社はAlexa Fluor 350、488、555、568、594、647および680アネキシンVコンジュゲート、アネキシンV APC、Biotin-X、FITC、Pacific Blue、およびPEコンジュゲートなどの最高レベルのアネキシンVコンジュゲート提供します。蛍光性の高いアネキシンVコンジュゲートは、アポトーシスの初期指標の1つであるホスファチジルセリンの外在化を研究するための迅速で信頼性の高い検出法を提供します。

アネキシンV Pacific Blueコンジュゲートはバイオレット励起性であり、バイオレットレーザーを備えた装置や、緑色または赤色蛍光色素を含むマルチカラー実験に最適です。

当社のアネキシンVコンジュゲートの利点：
•より明るいシグナルを得るためのInvitrogen Alexa FluorおよびeFluor色素に対するコンジュゲート
•利用可能なすべてのレーザー用のコンジュゲート
•独立した試薬または使いやすいキットとして利用可能

アポトーシス細胞を検出するためのアネキシンV染色は、生細胞および組織でのみ可能です。サンプルを染色後に固定する場合は、シグナルの一時的な保持を実現するために特定の条件が必要です。これには、アルコールを含まないアルデヒドベースの固定法の使用、Ca2+を含むバッファーの使用、界面活性剤／界面活性剤（洗剤）の回避などが挙げられます。また、アポトーシスアッセイにおけるホスファチジルセリンとアネキシンVとの結合を促進する濃縮アネキシン結合バッファーもご用意しています。

For Research Use Only. Not for use in diagnostic procedures.

仕様

色Red

概要アネキシンV、Alexa Fluor 594コンジュゲート

励起／発光590／617

フローサイトメーターレーザーライン532

使用対象 (装置)フローサイトメーター

キット内容アネキシンV、Alexa Fluor 594コンジュゲートのバイアル1本を含みます。

反応数100

製品タイプアネキシンVコンジュゲート

数量500 μL

出荷条件湿氷

コンジュゲートAlexa Fluor 594

Unit SizeEach

組成および保存条件

冷蔵庫（2℃～8℃）に保存し、遮光してください。

よくあるご質問（FAQ）

I want to study apoptosis using an Annexin V conjugate, but with adherent cells via microscopy instead of flow cytometry. Can this be done?

It has been done, but we don‘t recommend it. Both healthy cells and apoptotic cells possess phosphatidylserine on the cell surface, which can be detected with Annexin V, but apoptotic cells have significantly more of it. You can easily tell the difference between these two populations with flow cytometry, because flow cytometers are more sensitive and have a higher throughput. But with a microscope, you cannot always tell the difference, especially for adherent cells. Instead, for microscopy, we recommend a different technique, such as detecting caspases with CellEvent Caspase Detection Reagents.

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

I trypsinized my adherent cells and labeled with annexin V, and now my flow data is showing a high percentage of apoptotic cells even for control, untreated cells. What is the problem?

Trypsinization or mechanical scraping of cells temporarily disrupts the plasma membrane, allowing annexin V to bind phosphatidylserine on the cytoplasmic surface of the cell membrane and thus leading to false positive staining. Allow the cells to recover for about 30 minutes in optimal cell culture conditions and medium after trypsinizing/scraping so that they can recover their membrane integrity before staining. For lightly adherent cell lines, such as HeLa and NIH 3T3, another option is to use non-enzyme treatments like Gibco Cell Dissociation Buffer (Cat. No. 13151014).

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

Can I detect annexin V staining in an imaging assay?

Annexin V staining is not typically used in imaging experiments; it is a better reagent for flow cytometry analysis. All cells will stain to some extent, so it can be difficult to distinguish a relatively bright annexin V-stained cell from a dimmer non-apoptotic cell. Caspase activation, detected using our CellEvent Caspase 3/7 or Image-iT LIVE Caspase detection kits, is a better method for detecting apoptosis in an imaging assay.

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

When should I stain adherent cells with annexin V for flow cytometric analysis? Before or after I trypsinize them?

Trypsinize first and then allow the cells to recover about 30 minutes in optimal cell culture conditions and medium before staining with annexin V conjugates. Trypsinization or mechanical scraping of cells temporarily disrupts the plasma membrane, allowing for annexin V to bind phosphatidylserine on the cytoplasmic surface of the cell membrane and thus leading to false positive staining. For lightly adherent cell lines such as HeLa and NIH 3T3, you could use a less harsh (non-enzymatic) dissociation product like Gibco Cell Dissociation Buffer (Cat. No. 13151014).

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

Can I fix my cells after annexin V labeling?

Annexin V staining is best analyzed on live cells. If you need to fix your cells for analysis, then fix in 3.7% formaldehyde in PBS containing calcium and magnesium to maintain binding during fixation. The signal will not be retained after permeabilization, thus annexin V staining is not compatible with internal antibody labeling.

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

View all Annexin V Conjugates for Apoptosis Detection FAQs

引用および参考文献 (14)

引用および参考文献

Abstract

Caspase-mediated cleavage of the stacking protein GRASP65 is required for Golgi fragmentation during apoptosis.

Authors:Lane JD, Lucocq J, Pryde J, Barr FA, Woodman PG, Allan VJ, Lowe M

Journal:J Cell Biol

PubMed ID:11815631

'The mammalian Golgi complex is comprised of a ribbon of stacked cisternal membranes often located in the pericentriolar region of the cell. Here, we report that during apoptosis the Golgi ribbon is fragmented into dispersed clusters of tubulo-vesicular membranes. We have found that fragmentation is caspase dependent and identified GRASP65 ... More

A novel role for microtubules in apoptotic chromatin dynamics and cellular fragmentation.

Authors:Moss DK, Betin VM, Malesinski SD, Lane JD

Journal:J Cell Sci

PubMed ID:16723742

'Dramatic changes in cellular dynamics characterise the apoptotic execution phase, culminating in fragmentation into membrane-bound apoptotic bodies. Previous evidence suggests that actin-myosin plays a dominant role in apoptotic cellular remodelling, whereas all other cytoskeletal elements dismantle. We have used fixed cells and live-cell imaging to confirm that interphase microtubules rapidly ... More

Distinct phosphoinositide 3-kinases mediate mast cell degranulation in response to G-protein-coupled versus FcepsilonRI receptors.

Authors:Windmiller DA, Backer JM

Journal:J Biol Chem

PubMed ID:12529321

'Phosphoinositide (PI) 3-kinases are critical regulators of mast cell degranulation. The Class IA PI 3-kinases p85/p110beta and p85/p110delta but not p85/p110alpha are required for antigen-mediated calcium flux in RBL-2H3 cells (Smith, A. J., Surviladze, Z., Gaudet, E. A., Backer, J. M., Mitchell, C. A., and Wilson, B. S. et al., ... More

Cholesterol-induced apoptotic macrophages elicit an inflammatory response in phagocytes, which is partially attenuated by the Mer receptor.

Authors:Li Y, Gerbod-Giannone MC, Seitz H, Cui D, Thorp E, Tall AR, Matsushima GK, Tabas I

Journal:J Biol Chem

PubMed ID:16380374

'Macrophage apoptosis and the ability of phagocytes to clear these apoptotic cells are important processes in advanced atherosclerosis. Phagocytic clearance not only disposes of dead cells but usually elicits an anti-inflammatory response. To study this process in a model of advanced lesional macrophage death, macrophages rendered apoptotic by free cholesterol ... More

CD45-mediated fodrin cleavage during galectin-1 T cell death promotes phagocytic clearance of dying cells.

Authors:Pang M, He J, Johnson P, Baum LG,

Journal:J Immunol

PubMed ID:19454697

'Disassembly and phagocytic removal of dying cells is critical to maintain immune homeostasis. The factors that regulate fragmentation and uptake of dying lymphocytes are not well understood. Degradation of fodrin, a cytoskeletal linker molecule that attaches CD45 to the actin cytoskeleton, has been described in apoptotic cells, although no specific ... More

View all Annexin V Conjugates for Apoptosis Detection citations