A片粗大的内捧猛烈进出AVV,国产成人精品一区二区A片带套,久久久久久A片免费播放,无码人妻精一区二区三区

產(chǎn)品詳情
  • 產(chǎn)品名稱(chēng):Swant

  • 產(chǎn)品型號(hào):
  • 產(chǎn)品廠商:Swant
  • 產(chǎn)品文檔:
你添加了1件商品 查看購(gòu)物車(chē)
簡(jiǎn)單介紹:
SwantApply the streptavidine-biotin-peroxidase complex (diluted according to the suggestions of the supplier) or the Streptavidine-fluorescent complex in TBS with 10% carrier serum. Incubate for 1 to 2 hours at RT.Swant
詳情介紹:

Swant

  

國(guó)別:瑞士Swant

Swant  產(chǎn)品


  • 抗Ca2 +結(jié)合蛋白的抗體 Swant
  • 抗Ca2 +通道,Ca2 +交換劑和Ca2 +泵的抗體 Swant
  • 抗胰島素樣生長(zhǎng)因子的抗體 Swant
  • 針對(duì)神經(jīng)遞質(zhì)的抗體 Swant
  • 針對(duì)腎素 - 血管緊張素系統(tǒng)組分的抗體 Swant
  • 其他抗體 Swant
  • 純化蛋白 Swant


Antibodies to Calbindin D-28k, Calretinin, Parvalbumin, Calmodulin and to Na2+-Ca2+-exchangers, Ca2+ channels subunits, Ca2+ pumps, neurotransmitters, as well as their respective antigens.
Superb staining of subpopulation of neurons or glial cells in various species, including humans. Selective staining of various types of cancers.
Our mono- and polyclonal antibodies are of high titer and of high specificity. They can be used in immunohistochemistry and immunoblots at dilution of more than 1:5'000 (Avidin-Biotin-Method). The recombinant antigens have been purified by HPLC.
The products are supplied in lyophilized form and are accompanied by detailed product description. Method sheets can be found on this web-page.


Swant  Procedure for the immunolabelling of sections with rabbit antisera


Material


Free-floating cryostate or vibratome sections (40-80 μm) of fixed tissue* (4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4) or paraffin sections (3-5 μm) of tissue fixed with 10% unbuffered formalin.

0.1M Tris-buffered saline (TBS) pH 7.3.

SWant rabbit antiserum.

Biotinylated anti-rabbit IgG.

Streptavidin-peroxidase or Streptavidin conjugated to CY2, Cy3, Cy5, or other fluorescent dyes.

Peroxidase substrate (e.g. Diaminobenzidine(HCl) and H2O2).

Ethanol and Xylol.

Mounting medium (e.g. Eukitt for immunhistochemistry, Hydromount for immunofluorescence).

Method


Apply the SWant rabbit-antiserum diluted 1:1'000-1:5'000 (paraffin sections) or 1:5'000-1:10'000 (floating sections) in TBS with 10% carrier serum (e.g. calf or horse serum) and eventually 0.2% Triton-X 100 (particularly for vibratome sections). Incubate for 1 to 3 days at 4°C (on a shaker for free-floating sections, in a humid chamber for paraffin sections).

Rinse in TBS 3 x 5 min.

Apply biotinylated anti-rabbit IgG-biotin (diluted according to the suggestions of the supplier) in TBS with 10% carrier serum. Incubate at room temperature (RT) for 1 to 4 hours.

Rinse in TBS 3 x 5 min.

Apply the streptavidine-biotin-peroxidase complex (diluted according to the suggestions of the supplier) or the Streptavidine-fluorescent complex in TBS with 10% carrier serum. Incubate for 1 to 2 hours at RT.

Rinse in TBS 3 x 5 min.

The immunofluorescent labelling is terminated at this point and the section can be mounted on slides and coverslipped with an aqueous medium (e.g. Hydromount).

The immunohistochemical reaction is concluded by treating the section with a peroxidase substrate (e.g. Diaminobenzidine HCl / H2O2 ) under continuous microscopic observation.

Rinse in TBS 3 x 5 min.

Mount free floating sections on slides, eventually counterstain with cresyl-violet.

Dehydrate immunohistochemically treated sections with ethanol and xylol. Add mounting medium (Eukitt) and coverslip.

Note : in case of excessive background-staining, use higher dilutions of the SWant rabbit antiserum.


* Without prior fixation the highly soluble Ca2+-binding proteins are immediately lost during sectioning.



Procedure for the immunolabelling of sections with goat antisera


Swant  Material


Free-floating cryostate or vibratome sections (40-80 μm) of fixed tissue* (4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4) or paraffin sections (3-5 μm) of tissue fixed with 10% unbuffered formalin.

0.1M Tris-buffered saline (TBS) pH 7.3.

SWant goat antiserum.

Biotinylated anti-goat IgG.

Streptavidin-peroxidase or Streptavidin conjugated to CY2, Cy3, Cy5, or other fluorescent dyes.

Peroxidase substrate (e.g. Diaminobenzidine(HCl) and H2O2).

Ethanol and Xylol.

Mounting medium (e.g. Eukitt for immunhistochemistry, Hydromount for immunofluorescence).

Method


Apply the SWant goat-antiserum diluted 1:1'000-1:5'000 (paraffin sections) or 1:5'000-1:10'000 (floating sections) in TBS with 10% carrier serum (e.g. calf or horse serum) and eventually 0.2% Triton-X 100 (particularly for vibratome sections). Incubate for 1 to 3 days at 4°C (on a shaker for free-floating sections, in a humid chamber for paraffin sections).

Rinse in TBS 3 x 5 min.

Apply biotinylated anti-goat IgG-biotin (diluted according to the suggestions of the supplier) in TBS with 10% carrier serum. Incubate at room temperature (RT) for 1 to 4 hours.

Rinse in TBS 3 x 5 min.

Apply the streptavidine-biotin-peroxidase complex (diluted according to the suggestions of the supplier) or the Streptavidine-fluorescent complex in TBS with 10% carrier serum. Incubate for 1 to 2 hours at RT.

Rinse in TBS 3 x 5 min.

The immunofluorescent labelling is terminated at this point and the section can be mounted on slides and coverslipped with an aqueous medium (e.g. Hydromount).

The immunohistochemical reaction is concluded by treating the section with a peroxidase substrate (e.g. Diaminobenzidine HCl / H2O2 ) under continuous microscopic observation.

Rinse in TBS 3 x 5 min.

Mount free floating sections on slides, eventually counterstain with cresyl-violet.

Dehydrate immunohistochemically treated sections with ethanol and xylol. Add mounting medium (Eukitt) and coverslip.

Note: in case of excessive background-staining use higher dilutions of the SWant goat antiserum.


* Without prior fixation the highly soluble Ca2+-binding proteins are immediately lost during sectioning.

標(biāo)題:
內(nèi)容:
聯(lián)系人:
聯(lián)系電話:
Email:
公司名稱(chēng):
聯(lián)系地址:
 
 
注:1.可以使用快捷鍵Alt+S或Ctrl+Enter發(fā)送信息!
2.如有必要,請(qǐng)您留下您的詳細(xì)聯(lián)系方式!

滬公網(wǎng)安備 31011702004399號(hào)