產(chǎn)品名稱:RPMI Medium 1640(含雙抗) 培養(yǎng)基
產(chǎn)品型號(hào):31800-500
產(chǎn)品特點(diǎn):RPMI Medium 1640(含雙抗) 培養(yǎng)基中文名稱;RPMI Medium 1640生廠商:solarbio貨號(hào);31800規(guī)格:500ml保存條件: 2-8℃
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RPMI Medium 1640(含雙抗) 培養(yǎng)基
RPMI Medium 1640由GIBCO干粉配制,過濾滅菌。含雙抗、HEPES。保存期長,緩沖能力強(qiáng)。
細(xì)胞培養(yǎng)基既是培養(yǎng)細(xì)胞中供給細(xì)胞營養(yǎng)和促使細(xì)胞生殖增殖的基礎(chǔ)物質(zhì),也是培養(yǎng)細(xì)胞生長和繁殖的生存環(huán)境。
索萊寶公司生產(chǎn)的培養(yǎng)基精選進(jìn)口干粉,用超純?nèi)ルx子水配制,0.1um過濾而成,含雙抗,含Hepes。
RPMI Medium 1640(含雙抗) 培養(yǎng)基
平時(shí)研究用的細(xì)胞,有需要冷凍保存。冷凍的過程稱為凍存,把凍上的細(xì)胞化開的過程叫細(xì)胞復(fù)蘇。細(xì)胞復(fù)蘇是一簡單的試驗(yàn)操作,但操作中有許多需要注意的事項(xiàng),在實(shí)驗(yàn)操作中注意細(xì)小問題,才能使復(fù)蘇后的細(xì)胞狀態(tài)保持良好。
細(xì)胞復(fù)蘇實(shí)驗(yàn)準(zhǔn)備:
主要器材:一次性滴管、打火機(jī)、酒精燈、大鑷子、中鑷子、記號(hào)筆、廢液缸、封口膜、剪子。
主要試劑: PBS、培養(yǎng)液、消化酶(胰酶)、75%酒精、雙抗。
PBS配制:NaCL :4g KCL:0.1g Na2HPO4 :1.745g KH2PO4 :0.1g
三蒸水: 500mL,溶解后高壓滅菌。
培養(yǎng)基配制:5mL雙抗、50mL血清,加入培養(yǎng)基中。
細(xì)胞復(fù)蘇操作步驟:
1.佩戴眼鏡和手套,從液氮罐中取出安瓿或冷凍管。
2.迅速放入38℃水浴中,并不時(shí)搖動(dòng),在1分鐘內(nèi)使其*融化,然后在無菌下取出細(xì)胞。
3.在1000r/min速度下離心5~10分鐘,棄去上層液,加入適量培養(yǎng)液后接種于培養(yǎng)瓶中,接種濃度1×109/L,置37℃溫箱靜置培養(yǎng),次日更換一次培養(yǎng)液,繼續(xù)培養(yǎng),觀察生長情況。若細(xì)胞密度較高,及時(shí)傳代。或無需離心直接將細(xì)胞加入瓶中,并加入培養(yǎng)基貼壁培養(yǎng)12~24小時(shí)后,充去上清,換入新鮮培養(yǎng)基繼續(xù)培養(yǎng)。
細(xì)胞復(fù)蘇的注意事項(xiàng):
1.細(xì)胞復(fù)蘇時(shí)要注意融化凍存細(xì)胞的應(yīng)注意融化凍存細(xì)胞速度要快,可不時(shí)搖動(dòng)安瓿或冷凍管,使之盡快通過易受損的溫度段(-5~0℃)。
2.凍存液對(duì)細(xì)胞有毒性,解凍后必須用Dhanks洗兩遍才能移入培養(yǎng)瓶中培養(yǎng)。培養(yǎng)液中血清不能太少。
3.從液氮拿出來,以快速度丟入37度水浴,等細(xì)胞液剛剛化完取出,加培養(yǎng)液稀釋。這樣可以避免復(fù)蘇過程中細(xì)胞液中有冰晶的出現(xiàn),冰晶會(huì)破壞細(xì)胞膜及細(xì)胞內(nèi)部結(jié)構(gòu)的。
4.剛復(fù)蘇的細(xì)胞還是少折騰它好,細(xì)胞37°快速解凍后直接放入預(yù)熱的培養(yǎng)基。
5.DMSO在4度以下對(duì)細(xì)胞無毒,4度以上有毒;復(fù)蘇必須盡快除去。要記得慢凍速溶!
6.取細(xì)胞的過程中注意帶好防凍手套,護(hù)目鏡。細(xì)胞凍存管可能漏入液氮,解凍時(shí)凍存管中的氣溫急劇上升,可導(dǎo)致爆炸。
7.常溫下二甲基亞砜(DMSO)對(duì)細(xì)胞的毒副作用較大,因此,必須在1-2 min內(nèi)使凍存液*融化。如果復(fù)蘇溫度太低,會(huì)造成細(xì)胞的損傷,所以選擇40℃復(fù)蘇。8.貼壁細(xì)胞復(fù)蘇實(shí)驗(yàn)標(biāo)準(zhǔn)流程是將解凍后的細(xì)胞懸液行離心,以去除冷凍保護(hù)液DMSO對(duì)細(xì)胞的損傷,但是離心也會(huì)對(duì)剛復(fù)蘇的狀態(tài)欠佳的細(xì)胞產(chǎn)生損傷。也有的實(shí)驗(yàn)操作是將解凍后的細(xì)胞懸液先直接吹打均勻后分裝到培養(yǎng)瓶中進(jìn)行培養(yǎng),第二天換液。這可能使培養(yǎng)基中少量的DMSO對(duì)細(xì)胞造成損傷。
細(xì)胞復(fù)蘇后貼壁細(xì)胞較少的原意有哪些:
1.凍存細(xì)胞的時(shí)候是不是消化時(shí)間過長,這是一般人注意不到的地方,要知道太長的消化時(shí)間會(huì)使細(xì)胞復(fù)蘇時(shí)失去貼壁能力。
2.有可能是細(xì)胞凍存液的質(zhì)量,細(xì)胞凍存液的質(zhì)量不好也會(huì)導(dǎo)致細(xì)胞死亡。
3.凍存液的量加的是不是太多,ATCC推薦是不超過7%,大于5%,太多也不好。
4.凍存的時(shí)候是不是把DMSO混均勻,這個(gè)有一些影響,但不算太大。
5.凍存時(shí)溫度梯度是不是把握嚴(yán)格,很多人容易忘卻這個(gè)事情,因?yàn)檫@個(gè)東西流程長。
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