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当前位置: 首页 > 产品中心 > Sandwich_method_ELISA > Abbexa/Alkaline Phosphatase Live Detection Kit/50 µl/abx298024-50 µl
商品详细Abbexa/Alkaline Phosphatase Live Detection Kit/50 µl/abx298024-50 µl
Abbexa/Alkaline Phosphatase Live Detection Kit/50 µl/abx298024-50 µl
Abbexa/Alkaline Phosphatase Live Detection Kit/50 µl/abx298024-50 µl
商品编号: abx298024-50µl
品牌: Abbexa Ltd
市场价: ¥9570.00
美元价: 9570.00
产地: 美国(厂家直采)
公司:
产品分类: 夹心法ELISA
公司分类: Sandwich_method_ELISA
联系Q Q: 3392242852
电话号码: 4000-520-616
电子邮箱: info@ebiomall.com
商品介绍
Alkaline phosphatase (AP) is highly expressed in pluripotent stem cells, including embryonic stem cells (ESCs) and induced pluripotent stem cells (iPSCs). In the iPSCs induction process, the activation of AP is also necessary for successful reprogramming. In traditional AP detection methods, cells are fixed and cannot be used for further studies. This kit provides a fast, simple and sensitive method for AP detection without fixing the cells. The reagent is nontoxic to the cells, and the fluorescent signal will be discharged from the cells by exocytosis completely within two hours after removal of the staining solution, allowing the cell being used for following studies.
TargetAlkaline Phosphatase Live Detection Kit
StorageStore at -20 °C in the dark. Avoid repeated freeze/thaw cycles.
Kit Components
  • Alkaline Phosphatase Live Solution (500X): 20 µl or 50 µl
Material Required But Not Provided
  • 24-well plate (or similar)
  • DMEM/F12 preheated to 37 °C
  • Pipettes and pipette tips
  • Microcentrifuge tubes
  • 37 °C CO2 incubator
  • Fluorescence microscope
Directions for useAssay Procedure

The volumes of reagents in this protocol are based on a 24-well plate. For plates of other sizes, adjust the reagent volumes accordingly.

  1. Remove the growth medium from the cultures.
  2. Preheat DMEM/F12 to 37 °C. Wash with 500 µl of 37 °C DMEM/F12 for 3 minutes. Repeat the wash twice for a total of three times.
  3. Prepare the 1X working solution by diluting the 500X Alkaline Phosphatase Live Solution with DMEM/F12.
  4. Add 200 µl of 1X working solution directly to the cells and incubate in a 37 °C CO2 incubator for 30 minutes.
  5. Remove the working solution. Wash with 500 µl of DMEM/F12 for 3 minutes. Repeat the wash twice for a total of three times.
  6. Add 500 µl of DMEM/F12 to the cells and observe the results under a fluorescence microscope. Cells that express alkaline phosphatase (AP) are GFP positive and cells that do not express AP are GFP negative.
Notes
  1. Do not use pluripotent stem culture medium to dilute the 500X Alkaline Phosphatase Live Solution. Do not observe the result in pluripotent stem cell culture medium.
  2. Alkaline phosphatase is ubiquitously expressed in most cell types and is highly expressed in pluripotent stem cells. It is normal to observe dim staining in some somatic cells such as CHO cells, HeLa cells, placental cells etc.
  3. After removal of the dye from the media, fluorescently labelled cells lose their signal by exocytosis in 1.5-2 hours. It is recommended to observe the results within 1 hour after staining.
  4. Avoid freeze/thaw cycles. The working concentration can be increased if necessary.
AvailabilityShipped within 5-10 working days.
NoteThis product is for research use only. This product is shipped with dry ice.
Research Articles on Alkaline Phosphatase Live Detection Kit
品牌介绍
Isotype Control 同型对照 同型对照(Isotype Control),使用与一抗相同种属来源、相同亚型、相同剂量和相同的免疫球蛋白及亚型的免疫球蛋白,用于消除由于抗体非特异性结合到细胞表面而产生的背景染色。 同型对照 同型对照的主要目的是确定一抗的结合是特异性的,而不是非特异性的Fc受体或与其他蛋白的相互作用。还可以用来竞争性的结合抗体,与功能阻断抗体发挥同样的功能。 同型对照要与一抗的来源,Ig分型和标记完全一致。 如果一抗是多抗,可以用an normal serum(与一抗相同的正常血清) (must be the same species as primary antibody)。This control is easy to achieve and can be used routinely in immunohistochemical staining.这个可以咨询试剂商。同型对照为免疫荧光标记中的阴性对照。由于荧光标记单抗的组来源不同,应选用相同来源的未标记单抗作为同型对照来 调整背景染色。举个例子:比如检测一抗为单抗的mouse anti rat CD11b,clone OX-42 purified IgG,那么它的isotype 是mouse IgG2a, 所以可以用purified(纯化的) mouse IgG2a来做OX-42的同型对照(Isotype Control)。一般的的生物技术公司和国内的代理都有出售。 同型对照:是指与MoAb相同的、未免疫小鼠的免疫球蛋白亚类,若使用直接免疫荧光染色法,同型对照也应标记荧光色素,如IgG1 FITC、IgG2a、PE等。主要考虑了细胞的自发荧光、FC受体介导的抗体结合和非特异性抗体结合等影响因素。此外,同型对照与MoAb所标记的荧光 色素、浓度、F:P比值(标记的荧光色素与免疫球蛋白分子的比值)应该相同为最佳,这对准确设定阴性与阳性细胞的界标有重要意义,切忌使用与MoAb不相 匹配的同型对照,最好为同一实验室、采用相同工艺或方法制备(如同一品牌)的产品。