輪狀病毒(rotavirus,RV)純化方法�����,僅供參考
方法一
氯化銫密度梯度離心純化法(用密度梯度來做��,首先我們需要什么樣的轉(zhuǎn)頭����,角式的,或者是甩平轉(zhuǎn)頭�����,一般用甩平轉(zhuǎn)頭���。在準(zhǔn)備密度梯度時����,對病毒的浮力密度要清楚是多少�����,具體數(shù)字,然后我們才能知道用多大濃度的梯度介質(zhì)�。)
1、病毒濃縮
(1)PEG沉淀病毒:在收集到的病毒上清加入終濃度5%的PEG6000, 4℃攪拌過夜�����,10,000rpm, 4℃, 1.5小時離心�����,棄上清�����,用TNMC緩沖液(50mM Tris-Hcl pH7.5, 100mM Nacl, 10mM Cacl2,1mM Mgcl2 )懸浮沉淀�����;
(2)三氟三氯乙烷抽提:取PEG濃縮的病毒液���,加入等體積的三氟三氯乙烷(三氟三氯乙烷是有機(jī)溶劑�����,可以去除許多細(xì)胞中的雜質(zhì)(如脂類)�����,同時因為rotavirus沒有包膜��,所以能抵抗三氟三氯乙烷�����。)抽提一次�,12,000rpm, 4℃��,10min�,離心,收集水相,TNMC緩沖液10倍稀釋后�����,50,000rpm, 4℃, 1小時離心���,沉淀用TNMC緩沖液懸浮�����。
2�、CsCl密度梯度離心
取病毒液,與CsCl制成56%的乳化液��,裝入5ml梯度離心管中���,水平轉(zhuǎn)頭50,000rpm, 4℃, 22小時超速離心�。得三條乳白色的條帶�。分別收集離心所得的條帶,用TNMC緩沖液稀釋10-15倍���,50,000rpm, 4℃, 1.5小時��,離心去除CsCl�����,得到分離后較純的病毒��。
方法二
蔗糖密度梯度離心:
1�����、配制60%�、45%、30%���、15%的蔗糖(蔗糖M/水V)�,還有60%����、50%、40%�����、30%�、15%的蔗糖溶液也可以��。加熱溶解之后���,0.22UM濾器過濾�����,4度保存?zhèn)溆����,注意:一定要配的?zhǔn)確。
2���、蔗糖密度梯度離心管��,大和小兩種��。
3��、小管離心管����,每種蔗糖溶液加2~2.5ml�,依據(jù)你的病毒液體有多少。先加密度小的蔗糖溶液���,在加密度大的�����,依次類推���,加的時候要溫柔呵呵!用于加蔗糖梯度的注射器用干凈\高壓的玻璃注射器(2.5ML), 一次性塑料注射器密封性不好和注射器芯容易變形, 加蔗糖和樣品不準(zhǔn)����,針頭是比較長的,至少有10CM長,具體打電話問下試劑公司.
4�����、加蔗糖溶液有專門的針頭�����,比蔗糖離心管長����。
5��、要做這個試驗的時候�,提前把離心管洗干凈。
方法三
Preparation of Virions Containing Uncleaved VP4
1�����、Infect MA104 cells at a high MOI(3–10PFU/cell)with trypsin-activated virus.
2���、Wash the cell sheet several times with serum-free medium following adsorption.
3、Maintain the cells in trypsin-free medium containing 1μg/mL aprotinin or 0.5μg/mL leupeptin.
4�、Harvest the cells once the CPE has reached 70–80% (24 h post infection).
Purification of Triple-Layered Virions
1�����、Combine the lysate with an equal volume of trichlorotrifluoroethane, and homogenize the mixture with a Sorvall Omni-mixer for three 1min cycles on ice.
2���、Centrifuge the homogenates at low speed to separate the organic and aqueous phases (4100g for 10 min in a Sorvall GSA rotor at 4°C).
3、Pellet the virus particles from the aqueous phase by centrifugation at 90,000g in a Beckman (Palo Alto, CA) SW28 rotor or at 45,000g in a Beckman Type 19 rotor for 2h at 4°C.
4����、Resuspend the pellet in TBS, and add CsCl to the virus suspension to achieve a density of 1.370g/cm3, as determined by refractometry (see Note 7).
5、Centrifuge the mixture at 110,000g in a Beckman SW50.1 rotor for 20h at 4°C.
6���、Inspect the gradients in a darkened room with an inverted light source, to reveal two bands.
7���、Recover the virus from the gradient by puncturing the bottom of the centrifuge tube with a 21-gage needle, and collect drops containing TLPs and DLPs, respectively,into separate tubes.
8、Remove the CsCl by dialyzing the virus extensively against TBS at 4°C.
9����、Store the dialyzed samples at 4°C in the presence of 0.01% NaN3.
Tris-buffered saline(TBS): 8g NaCl, 0.38g KCl, 0.1g Na2HPO4, 1g dextrose,3g Tris-base, 0.1g MgCl2, 0.1g CaCl2. Dissolve in distilled H2O, adjust to pH 7.4 with HCl, and make up to 1L.
用完整的病毒作為抗原,做ELISA試劑的最低層����,不需要純化病毒。只需包被RV作檢測抗體之用��,這是間接法ELISA。細(xì)胞培養(yǎng)的病毒用包被緩沖液做1:40稀釋(病變出的好��,這個稀釋度就跑不了�����,我們實驗室做了若干年了)����,每孔100ul,過夜成了。如果不放心�,可以高速離心后再過G200柱,這個方法比超離方便多了�。病毒從凝膠空隙最早流出,而雜蛋白進(jìn)入孔內(nèi)出來的緩慢�。ELISA不需要太純的病毒。不知道是SA11還是Wa株����?前者病變非常典型,后者病變緩慢���,如果不放心1:40稀釋,可以用有限稀釋方法滴定抗原用量��。
