1. To a 10 ml centrifuge tube add 2 ml of defibrinated- or anticoagulant-treated blood and an equal volume of balanced salt solution (final volume 4 ml).

2. Mix the blood and buffer by inverting the tube several times or by drawing the mixture in and out of a pipette.

Procedure for isolation of mononuclear cells

1. Invert the Ficoll-Paque media bottle several times to ensure thorough mixing.

For withdrawal of Ficoll-Paque media by syringe:

Snap-off the polypropylene cap and insert the syringe needle through the septum (Fig 1).

For withdrawal of Ficoll-Paque media by pipette:

Remove the snap-off polypropylene cap. Lift the aluminum ring. Pull off the metal seal. Remove the silver ring.Remove the rubber closure. Using aseptic techniques, withdraw the required volume of Ficoll-Paque media.

2. Add Ficoll-Paque media (3 ml) to the centrifuge tube.

3. Carefully layer the diluted blood sample (4 ml) onto the Ficoll-Paque media solution (Fig 3).

Important: When layering the sample do not mix the Ficoll-Paque media solution and the diluted blood sample.

4. Centrifuge at 400 g for 30 to 40 min at 18ºC to 20°C (brake should be turned off).

5. Draw off the upper layer containing plasma and plaets using a sterile pipette, leaving the mononuclear cell layer undisturbed at the interface (Fig 4 and Fig 5). The upper layer, which contains the plasma, may be saved for later use.

6. Transfer the layer of mononuclear cells to a sterile centrifuge tube using a sterile pipette.

Washing the cell isolate

1. Estimate the volume of the transferred mononuclear cells. Add at least 3 volumes (~ 6 ml) of balanced salt solution to the mononuclear cells in the centrifuge tube.

2. Suspend the cells by gently drawing them in and out of a pipette.

3. Centrifuge at 400 to 500 × g for 10 to 15 min at 18°C to 20°C.

Note: A centrifugation at high speed increases the mononuclear cell recovery. However, if it is important to also get rid of plaets a lower centrifugation speed is recommended (60 to 100 × g).

4. Remove the supernatant.

5. Resuspend the mononuclear cells in 6 to 8 ml balanced salt solution.

6. Centrifuge at 400 to 500 × g (or 60 to 100 × g for removal of plaets) for 10 min at 18°C to 20°C.

7. Remove the supernatant.

8. Resuspend the cell pellet in media appropriate for the application.

Ficoll-Paque單個(gè)核細(xì)胞分離方法由紅榮微再翻譯整理。準(zhǔn)確詳情以及疑難解答等參見說明書。

GE淋巴細(xì)胞分離液是一種無菌、即用型的淋巴細(xì)胞分離液，根據(jù)外周血中各類細(xì)胞在密度梯度離心中呈現(xiàn)不同的密度梯度分布而將全血中的淋巴細(xì)胞等單個(gè)核細(xì)胞進(jìn)行分離。適用人外周血、骨髓和臍帶血的單個(gè)核細(xì)胞分離。與Ficoll-Paque PLUS不同的是，F(xiàn)icoll-Paque PREMIUM的生產(chǎn)是在嚴(yán)格控制環(huán)境下完成的, 生產(chǎn)條件符合ISO 13485標(biāo)準(zhǔn)，GMP認(rèn)證和美國(guó)藥典，可用于生產(chǎn)臨床級(jí)細(xì)胞治療相關(guān)產(chǎn)品。

訂購信息

品牌	貨號(hào)	產(chǎn)品描述	包裝
GE	17-1440-02	Ficoll-Paque PLUS,1.078 g/ml淋巴細(xì)胞分離液	6 × 100 ml
GE	17-1440-03	Ficoll-Paque PLUS,1.078 g/ml淋巴細(xì)胞分離液	6 × 500 ml
GE	17-5442-02	Ficoll-Paque PREMIUM,1.077 g/ml淋巴細(xì)胞分離液	6 × 100 ml
GE	17-5442-03	Ficoll-Paque PREMIUM,1.077 g/ml淋巴細(xì)胞分離液	6 × 500 ml
GE	17-5446-52	Ficoll-Paque PREMIUM 1.073,1.073 g/ml 淋巴細(xì)胞分離液	6 × 100 ml

咨詢GE Ficoll-Paque density gradient media 淋巴細(xì)胞分離液歡迎您致電華雅再生醫(yī)學(xué)旗艦公司：紅榮微再（上海）生物工程技術(shù)有限公司

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細(xì)胞治療

耗材

細(xì)胞凍存/細(xì)胞分離

細(xì)胞庫

干細(xì)胞（無血清）培養(yǎng)基

血清及替代物/細(xì)胞因子

抗體/蛋白質(zhì)

核酸分析/測(cè)序/蛋白組學(xué)

小型儀器設(shè)備

檢測(cè)試劑

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生長(zhǎng)因子/細(xì)胞因子

PCR試劑耗材

NGS測(cè)序試劑耗材

Ficoll-Paque單個(gè)核細(xì)胞分離方法