SYTOX™ AADvanced™ Dead Cell Stain Kit
SYTOX™ AADvanced™ Dead Cell Stain Kit
Invitrogen™

SYTOX™ AADvanced™ Dead Cell Stain Kit

SYTOX™ AADvanced™ Dead Cell Stain(S10274、S10349)は、フローサイトメトリーで一般的な488 nm青色レーザーを使用した死細胞の検出および細胞周期の分析用の新しい高親和性核酸染色剤です詳細を見る
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製品番号(カタログ番号)数量
S10274500 Reactions
S10349100反応
製品番号(カタログ番号) S10274
価格(JPY)
89,200
Each
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数量:
500 Reactions
SYTOX™ AADvanced™ Dead Cell Stain(S10274、S10349)は、フローサイトメトリーで一般的な488 nm青色レーザーを使用した死細胞の検出および細胞周期の分析用の新しい高親和性核酸染色剤です。この色素は7-AADとスペクトル的に類似しますが、取り込み速度が大きく、CVは比較的低値にあります。SYTOX™ AADvanced™ Dead Cell Stainは、7-AADよりも効率的に細胞に浸透し、生細胞と死細胞の分離を向上させます。SYTOX™ AADvanced™ Dead Cell Stainは、RNase処理と組み合わせることで、固定細胞と併用してDNA含有量を分析することもできます。SYTOX™ AADvanced™ Dead Cell Stain Kitには、乾燥した色素と無水DMSOのバイアルが含まれており、安定した保存期間を提供します。

フローサイトメトリー用のすべての固定不可能生存率色素の選択ガイドをご覧ください。
研究用にのみ使用できます。診断用には使用いただけません。
仕様
細胞透過性Impermeant
概要SYTOX™ AADvanced™ Dead Cell Stain Kit
検出法蛍光
染色剤タイプSYTOX™ AADvanced™
形状固体
フォーマットチューブ
数量500 Reactions
出荷条件室温
溶解性DMSO(ジメチルスルホキシド)
細胞内局在核、核酸
Red
Emission546⁄647
Excitation Wavelength Range546 nm
使用対象(アプリケーション)生存率アッセイ
使用対象 (装置)フローサイトメーター
製品ラインMolecular Probes、SYTOX
製品タイプDead Cell Stain Kit
Unit SizeEach
組成および保存条件
SYTOX™ AADvanced™死細胞染色液 x 5バイアル、500 μLジメチルスルホキシド(DMSO)。 遮光し、≤-20℃で保存。

よくあるご質問(FAQ)

How do SYTO dyes bind to DNA?

The binding mode of SYTO nucleic acid stains is unknown. However, the behavior of these and related nucleic acid dyes suggests the following binding properties:

1.They appear to contact the solvent (suggested by sensitivity to salt, divalent cations, and in particular, SDS) and thus are likely to have contacts in the grooves.
2.All SYTO dyes appear to show some base selectivity and are thus likely to have minor groove contacts.
3.They can be removed from nucleic acid via ethanol precipitation; this characteristic is not shared by ethidium bromide and other intercalators. Likewise, the dyes are not removed from nucleic acid via butanol or chloroform extraction. These extraction methods do remove ethidium bromide from nucleic acid. 4. SYTO binding is not affected by nonionic detergents.
5. SYTO dyes are not quenched by BrdU, so they do not bind nucleic acids in precisely the same way as Hoechst 33342 and DAPI ((4′,6-diamidino-2-phenylindole).

SYBR Green I has shown little mutagenicity on frameshift indicator strains, indicating that it isn't likely to strongly intercalate.

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

I am using SYTOX AAdvanced as a dead cell stain, but all of my cells are labeling even though I am certain that they are supposed to be alive. These are adherent cells that I have trypsinized. Why am I getting false-dead signals?

SYTOX AAdvanced labels only dead cells because it is a cell impermeant dye. The dye can only enter cells that have a compromised plasma membrane. Trypsinization may cause temporary disruption of the plasma membrane, sufficient to allow staining with a cell impermeant dye. You can reduce the “false-dead” problem by either reducing the amount of trypsin and/or reduce the incubation time for trypsinization or use a gentler dissociation reagent such as TrypLE Express, TrypLESelect reagents, or Versene. After trypsinization, wash well, and if possible, allow a recovery time in normal culture media before staining with any of the SYTOX dyes.

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

My cell cycle data show a single peak, not a proper cell cycle profile. How can I fix this?

There are several factors that contribute to the quality of the cell cycle profile. Cell number, dye concentration, incubation temperature, incubation time, flow rate (on a traditional flow cytometer utilizing hydrodynamic focusing), total number of cells acquired, elimination of dead cells, and removal of aggregates from data analysis should all be considered when analyzing the cell cycle.

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