| 產(chǎn)品名稱 |
RKO-E6 |
| 商品貨號 |
MZ-0248 |
| 中文名稱 |
人結(jié)腸癌轉(zhuǎn)基因細(xì)胞 |
| 細(xì)胞數(shù)量 |
1*10^6 |
| 組織來源 |
colon |
| 細(xì)胞種屬 |
Homo sapiens, human |
| 細(xì)胞污染 |
HIV-1���、 HBV���、HCV、支原體��、細(xì)菌、酵母和真菌檢測陰性�。 |
| 生長特性 |
adherent |
| 培養(yǎng)基 |
MEM+10% FBS+1% P/S |
| 形態(tài)特征 |
epithelial |
| 傳代方法 |
1:3-1:10 |
| 培養(yǎng)條件 |
Atmosphere: Air, 95%; CO2, 5%。Temperature: 37℃ |
| 細(xì)胞描述 |
The cells contain a stably integrated human papilloma virus(HPV) E6 oncogene under control of the cytomegalovirus(CMV) promoter. The HPV E6 oncogene causes a decrease in normal p53 levels and functions.The RKO-E6 cell line lacks appreciable functional p53.Disruption of normal p53 function in human colon carcinoma RKO cells with the human papillomavirus E6 oncoprotein results in reduced repair of u.v.-induced DNA damage and also loss of induced repair following cellular u.v.- irradiation.RKO cells contain wild-type p53 but lack endogenous human thyroid receptor nuclear receptor(h-TRbeta1). The level of p53 protein is higher in RKO cells than in RKO-E6 cells.The RKO-E6 cell line can be used together with its parental cell line, RKO to investigate the effects of p53 loss on cellular parameters such as p53 mediated transcription and apoptosis. |
| 細(xì)胞傳代步驟 |
如果細(xì)胞密度達(dá)80%-90%��,即可進(jìn)行傳代培養(yǎng)�。1. 棄去培養(yǎng)上清,用不含鈣���、鎂離子的PBS潤洗細(xì)胞1-2次���。2. 加2ml消化液(0.25%Trypsin-0.53mM EDTA)于培養(yǎng)瓶中,置于37℃培養(yǎng)箱中消化1-2分鐘���,然后在顯微鏡下觀察細(xì)胞消化情況��,若細(xì)胞大部分變圓并脫落���,迅速拿回操作臺,輕敲幾下培養(yǎng)瓶后加少量培養(yǎng)基終止消化��。3. 按6-8ml/瓶補(bǔ)加培養(yǎng)基��,輕輕打勻后吸出��,在1000RPM條件下離心4分鐘,棄去上清液���,補(bǔ)加1-2mL培養(yǎng)液后吹勻��。4. 將細(xì)胞懸液按1:2到1:5的比例分到新的含8ml培養(yǎng)基的新皿中或者瓶中 |
| 復(fù)蘇細(xì)胞步驟 |
將含有1mL細(xì)胞懸液的凍存管在37℃水浴中迅速搖晃解凍��,加入4mL培養(yǎng)基混合均勻��。在1000RPM條件下離心4分鐘��,棄去上清液��,補(bǔ)加1-2mL培養(yǎng)基后吹勻���。然后將所有細(xì)胞懸液加入培養(yǎng)瓶中培養(yǎng)過夜(或?qū)⒓?xì)胞懸液加入10cm皿中��,加入約8ml培養(yǎng)基�,培養(yǎng)過夜)。第二天換液并檢查細(xì)胞密度��。 |
| 細(xì)胞凍存步驟 |
:待細(xì)胞生長狀態(tài)良好時��,可進(jìn)行細(xì)胞凍存�。下面T25瓶為例�;1.細(xì)胞凍存時��,棄去培養(yǎng)基后���,PBS清洗瓶底1-2次后加入1ml胰酶�,細(xì)胞變圓脫落后��,加入2ml完全培養(yǎng)基終止消化��,可使用血球計(jì)數(shù)板計(jì)數(shù)�。2.1000RPM離心5分鐘去掉上清。用血清重懸浮��,加DMSO至最終濃度為10%��。加入DMSO后迅速混勻���,按每1ml的數(shù)量分配到凍存管中��,注意凍存管做好標(biāo)識�。本公司按每個凍存管細(xì)胞數(shù)目大于1X106個細(xì)胞凍存�。3.將凍存管置于程序降溫盒中,放入-80度冰箱,至少2個小時以后轉(zhuǎn)入液氮灌儲存��。記錄凍存管位置以便下次拿取�。 |
| 細(xì)胞凍存 |
Freeze medium: 50% basal medium+40% FBS+10%.DMSOStorage temperature: liquid nitrogen vapor phase |
| 細(xì)胞運(yùn)輸 |
干冰運(yùn)輸(2ml凍存管)或活細(xì)胞運(yùn)輸(T25細(xì)胞瓶) |
