細(xì)胞培養(yǎng)進(jìn)口血清進(jìn)口胎牛血清進(jìn)口新生牛血清進(jìn)口豬血清馬血清- 支原體檢測盒及標(biāo)準(zhǔn)品常規(guī)PCR檢測試劑盒熒光定量PCR檢測(qPCR法)支原體DNA提取靈敏度標(biāo)準(zhǔn)品(方法驗(yàn)證用)特異性標(biāo)準(zhǔn)品(方法驗(yàn)證用)PCR定量標(biāo)準(zhǔn)品(可用于方法驗(yàn)證)
支原體祛除試劑細(xì)胞中支原體祛除環(huán)境支原體祛除水槽支原體祛除
干細(xì)胞培養(yǎng)基- DNA/RNA污染祛除DNA/RNA污染祛除試劑DNA污染監(jiān)測
- RNA病毒研究試劑RNA病毒檢測試劑盒病毒RNA提取
- PCR儀器及配套產(chǎn)品DNA污染監(jiān)測祛除PCR/qPCR儀性能檢查PCR試劑PCR試劑盒PCR預(yù)混液(凍干粉)熱啟動聚合酶MB Taq DNA
- 微生物PCR檢測食品檢測類產(chǎn)品食品微生物檢測細(xì)菌PCR檢測
細(xì)胞培養(yǎng)進(jìn)口血清
支原體祛除試劑
干細(xì)胞培養(yǎng)基
- 細(xì)胞培養(yǎng)進(jìn)口血清進(jìn)口胎牛血清進(jìn)口新生牛血清進(jìn)口豬血清馬血清
- 支原體檢測盒及標(biāo)準(zhǔn)品常規(guī)PCR檢測試劑盒熒光定量PCR檢測(qPCR法)支原體DNA提取靈敏度標(biāo)準(zhǔn)品(方法驗(yàn)證用)特異性標(biāo)準(zhǔn)品(方法驗(yàn)證用)PCR定量標(biāo)準(zhǔn)品(可用于方法驗(yàn)證)
- 支原體祛除試劑細(xì)胞中支原體祛除環(huán)境支原體祛除水槽支原體祛除
- 干細(xì)胞培養(yǎng)基
- DNA/RNA污染祛除DNA/RNA污染祛除試劑DNA污染監(jiān)測
- RNA病毒研究試劑RNA病毒檢測試劑盒病毒RNA提取
- PCR儀器及配套產(chǎn)品DNA污染監(jiān)測祛除PCR/qPCR儀性能檢查PCR試劑PCR試劑盒PCR預(yù)混液(凍干粉)熱啟動聚合酶MB Taq DNA
- 微生物PCR檢測食品檢測類產(chǎn)品食品微生物檢測細(xì)菌PCR檢測
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比較研究胎牛血清和馬血清對初級馬支氣管成纖維細(xì)胞的生長和分化的影響2016-09-23 13:25
從消化支氣管組織細(xì)胞產(chǎn)量是一致的。在這兩種培養(yǎng)條件,EBF用臺盼藍(lán)染色和活細(xì)胞的百分率是相似的,通常>95%。下倒光鏡分析,觀察細(xì)胞壞死或凋亡的細(xì)胞沒有顯著的證據(jù)。對于細(xì)胞形態(tài),EBF在DMEM中培養(yǎng),用10%FBS的似乎是通常扁平和紡錘形(具有均勻的細(xì)胞質(zhì))在幾個星期的通道相比EBF在DMEM中培養(yǎng),用10%的HS(圖1的A)。 在FBS的培養(yǎng)基,EBF生長在生長表面只有松散的細(xì)胞-細(xì)胞接觸,直到達(dá)到匯合,然后形成了仍然是典型的成纖維細(xì)胞單層,直到通道15道之間EBF緊平行線16-20開始改變其形態(tài):細(xì)胞大,平坦和更多邊形的形狀,具有大,異質(zhì)核。同時,細(xì)胞生長迅速降低和細(xì)胞存活率降低。與此相反,EBF在HS的存在下培養(yǎng)的表現(xiàn)出內(nèi)培養(yǎng)2天改變形態(tài)學(xué)變化;細(xì)胞小,形狀在細(xì)胞質(zhì)顆粒劑般黑暗的結(jié)構(gòu)(圖結(jié)合更緊湊1C)。 此外,細(xì)胞生長集群和鏈條,未能在一周內(nèi)達(dá)到匯合。EBF的這種形態(tài)行為這種文化條件下看到,直到第7代,但此后,EBF未能定期增殖,并在自己的生存能力(通道9)下降。在這兩種培養(yǎng)條件下,最EBF(>99%)為陽性波形蛋白,但與細(xì)胞質(zhì)內(nèi)的培養(yǎng)基含有FBS的(圖更特性絲狀結(jié)構(gòu)1B)的比在HS(圖的存在1D). 總之,血清中除基礎(chǔ)EBF培養(yǎng)基提高EBF分化成肌成纖維細(xì)胞,而這些發(fā)現(xiàn)開發(fā)出模擬體內(nèi)的生理過程,并研究氣道疾病的機(jī)制和重塑體外成纖維細(xì)胞培養(yǎng)模型有用。 英文原文: Comparative study of the effects of fetal bovine serum versus horse serum on growth and differentiation of primary equine bronchial fibroblasts
Primary EBF were cultured on non-collagen coated flasks without serum or in the presence of fetal bovine serum (FBS) or horse serum (HS) or in serum depleted medium. EBF cultured in serum-free basal media and those serum deprived were not able to proliferate and even exhibited considerable cell death. In media containing FBS or HS, proliferation of the cells was reproducible between different primary cultures and cells demonstrated expression of vimentin. Large variations were found in the ability of FBS and HS to support growth and differentiation of EBF in monolayer culture. Indications of growth-promoting actions, increasing passage number as well as maintaining fibroblast morphology were found rather in FBS than in HS. EBF culturing in HS needed longer doubling and confluence time. The protein content of the cell pellets was higher in EBF cultured in medium containing HS than FBS. Alpha-smooth muscle actin seemed to be less expressed in EBF cultured in medium containing FBS than those in HS.
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