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當前位置:上海富雨生物科技有限公司>>細胞庫 / 細胞培養>>細胞株>> hct116/FU人結腸癌氟尿
產品名稱:hct116/FU人結腸癌氟耐藥株、hct116/FU人結腸癌氟耐藥株、hct116/FU人結腸癌氟耐藥株、hct116/FU人結腸癌氟耐藥株;
細胞系特征 | ||
細胞株名稱:HCT116/FU人結腸癌耐氟細胞株 種屬:人 組織來源:結腸癌 生長特性:貼壁生長 形態特征:上皮細胞 微生物及支原體檢測:陰性 安全性:所有腫瘤和病毒轉染的細胞均視為有潛在的生物危害性,必須在二級生物安全臺內操作,并請注意防護,所有廢液及接觸過此細胞的器皿需高壓滅菌后方能丟棄。 | ||
培養條件:
| 培養基:90%RPMI-1640+10%胎牛血清+2ug/ml FU 血清我們推薦用: GIBCOFBS-10099-141或HYCLONEFBS-SH30084.03。 培養條件:37.0C carbon dioxide(CO2),5% | |
傳代方法:
| 收到細胞后,在倒置鏡下(是在4X物鏡)觀察整個細胞生長情況。 (一)如果細胞未長滿,用75%酒精噴灑整個瓶消毒后放到超菌臺內,嚴格無菌操作,打開細胞培養瓶,吸出培養液,換 10ml新鮮培養液后繼續培養。 (二)如果細胞已長滿,即可進行傳代培養。具體步驟如下: 1. 棄去培養液,用PBS(不含鈣,鎂離子)洗1-2次。 2. 加0.7-1ml消化液(0.25%Trypsin-0.53mM EDTA)于培養瓶中,用力拍打瓶壁,期間每隔 5-10s放到顯微鏡下觀察,直至50-70%的細胞脫落后,加入2ml 以上培養基中止消化。 3. 按6-8ml/瓶補加培養基,輕輕打勻后吸出一半,分到新的培養瓶中。如果沒有特別說明,收到細胞后的次傳代一般是一傳二。 注:1、觀察細胞在低倍鏡(4或5X物鏡)下進行,否則不能準確判斷細胞的傳代密度。看細胞的形態請在10X或20X物鏡下。 2、瓶中運輸培養基不能重復再用,請換用加雙抗的新培養基,細胞凍存后,培養基中可不加任何抗生素。 3、有些細胞貼壁不牢,如發現貼壁細胞有脫落,可離心吹打后接種到新瓶內。 4、收到細胞后,若發現培養瓶破損、有液溢出及細胞有污染,請及時與我們聯系。..
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凍存方法: | 凍存液:90%胎牛血清,10%DMSO 儲存:液氮儲存 |
In addition to participating in the regulation of T cell proliferation, survival, and TCR
signaling,autophagy has recently been shown to control CD8+ T cell memory generation
[ 10, 84]. Mice bearing Atg7-deficient CD8+ T cells showed impaired memory formation
using influenza or murine cytomegalovirus models, as well as diminished recall responses to secondary influenza infection [84]. Similarly, in a granzyme-Cre Atg7fl/fl mouse model,
CD8+ T cells had cell-intrinsic defects in memory formation in response to lymphocytic
Figure 2. Roles of autophagy in T cells
Engagement of the TCR and CD28 signaling pathways is required for full activation of T cells, which can be further augmented by signaling through the IL-2r. Autophagy is
maintained at basal levels inna?ve and resting T cells and the cargo of autophagosomes
largely consists of organelles, such as mitochondria (1), which is an important quality
control mechanism. TCR- and IL-2r-signaling induce autophagy. Upon activation the cargo nature switches to mostly cytosolic components, and activation-induced degradation of
specific proteins (p27, caspases, Bim or Bcl10) has been described to control proliferation, survival and activation. Important roles of Autophagy have been reported in the regulation of cell homeostasis (2); TCR signaling transduction (3); the breakdown of macromolecules to recycle cellular building blocks and generate signaling metabolites (4); and the regulation of T cell metabolism (5). In addition, macroautophagy has been shown to be necessary for
CD4+ T cell activation, cell survival, and proliferation (6), differentiation of specific CD4+ T helper sucdfts, (7), enforcing Treg lineage stability (8), and for generation of CD8+
memory T cells (9).
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