SYTOX™ Green 核酸染料 - 5 mM 的 DMSO 溶液
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SYTOX™ Green 核酸染料 - 5 mM 的 DMSO 溶液
Invitrogen™

SYTOX™ Green 核酸染料 - 5 mM 的 DMSO 溶液

SYTOX® Green 核酸染料是一种极佳的绿色荧光核和染色体复染剂,不可透过活细胞,从而可作为细胞群中死细胞的有效指示剂。还可以室温下稳定的即用型溶液形式提供:NucGreen Dead 488 Ready Probes 试剂。查看其他了解更多信息
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货号数量
S7020250 μL
货号 S7020
价格(CNY)
3,503.00
飞享价
Ends: 31-Dec-2025
4,747.00
共减 1,244.00 (26%)
Each
添加至购物车
数量:
250 μL
价格(CNY)
3,503.00
飞享价
Ends: 31-Dec-2025
4,747.00
共减 1,244.00 (26%)
Each
添加至购物车
SYTOX® Green 核酸染料是一种极佳的绿色荧光核和染色体复染剂,不可透过活细胞,从而可作为细胞群中死细胞的有效指示剂。

还可以室温下稳定的即用型溶液形式提供:NucGreen Dead 488 Ready Probes 试剂
查看其他 Ready Probes 即用型成像试剂及附件 ›

 不可透过活细胞
 激发/发射:504/523 nm
 与 488 nm 氩离子激光配合使用
 适用于哺乳动物细胞以及革兰氏阳性和革兰氏阴性细菌

活力测定简便
SYTOX® Green 可使用流式细胞仪、荧光显微镜、荧光计或荧光微孔板酶标仪快速测定细胞活力。其不会穿过完整的细胞膜,但可轻易穿透受损的细胞膜,而这正是死细胞的特征。由于结合核酸后,荧光会增强 >500 倍,所以使用 SYTOX® Green 与死细胞短暂孵育后,在通过 488 nm 氩离子激光或任何其他 450–490 nm 的光源激发时,会产生明亮的绿色荧光,发射峰为 523 nm。死细胞产生的信号非常明亮,因此 SYTOX® Green 不仅特别适用于确定哺乳动物细胞的活力,还可用于革兰氏阳性和革兰氏阴性细菌的活力测定。

Invitrogen 系列细胞活力染料和检测
适用于死细胞的 SYTOX® 染色剂有多种颜色可供选择,包括红色、蓝色和橙色。此外,Invitrogen 还将 SYTOX® 染色剂用于多种细胞凋亡、细胞活性和代谢测定。

仅供科研使用。不适用于任何动物或人类治疗或诊断用途。

相关链接
•  了解更多有关所有 SYTOX® 产品的信息。

仅供科研使用。不可用于诊断程序。
规格
颜色绿色
检测方法荧光
染料类型细胞通透性
发射523 nm
激发波长范围504 nm
适用于(设备)流式细胞仪
形式溶液
产品规格
产品线SYTOX
数量250 μL
运输条件室温
容积(公制)250 μL
标签类型荧光
产品类型核酸染色剂
亚细胞定位细胞核,核酸, Nucleus
Unit SizeEach
内容与储存
在冷柜(-5°C 至 -30°C)中避光储存。

常见问题解答 (FAQ)

这些染料如何与DNA结合?

SYTO核酸染料的结合方式尚不清楚。但是,SYTO以及相关的核酸染料具有以下结合特性:

1.它们与一些溶剂结合(通过对盐、二价阳离子的敏感性,特别是SDS),因此,它们可能结合到DNA沟槽处。
2.所有SYTO染料都表现出一些碱基选择性,因此,它们可能结合到DNA小沟处。
3.通过乙醇沉淀可从核酸中去除SYTO染料;溴化乙锭和其他嵌入剂不具有此特性。同样,丁醇和氯仿提取不能从核酸中去除SYTO染料,但能够去除溴化乙锭。
4.SYTO 结合不受非离子去垢剂的影响。
5.SYTO染料不会被BrdU淬灭,因此,SYTO染料与核酸的结合方式不同于Hoechst 33342和DAPI(4',6-二脒基-2-苯基吲哚)。

SYBR Green I对移码指示菌几乎没有致突变性,证明其不大可能是强嵌入剂。

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 need to mount my Qdot secondary-labeled tissue samples in HistoMount mounting medium, but my Qdot 705 conjugate overlaps with your Qnuclear Deep Red nuclear label. What other nuclear label would you recommend, that is compatible with HistoMount mounting medium?

We recommend using SYTOX Green stain, which you can image using a FITC filter and we have shown to be compatible with HistoMount mounting medium. Some have used DAPI, but there have been some issues with slight quenching and spectral shifting of DAPI into green or even red wavelengths.

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.