鲐鱼鱼精中5_脱氧核苷酸的分离工艺

论述了用桔青霉PenicilliumcitrinumM71菌株,经液体培养制得的5＇-磷酸二酯酶降解鲐鱼鱼精DNA成5＇-脱氧核苷酸的分离工艺.分离采用201×8阴离子交换树脂,具体条件为柱床高l05mm,柱床直径45mm,样品浓度213mg@mL-1,洗脱流速0.5mL@cm-2@min-1.分离结果表明,采用0.005MHCl+0.04MNaCl作洗脱刺,流速为0.7mL@cm-2@min-1时,四种5'-脱氧核苷酸组分能完全被洗脱下来,且呈一个大峰,同其它成分分开,再先后采用0.0018MHCl、0.0028MHCl、0.036MNaCl(pH6.0)、0.005MHCl+0.02MNaCl作洗脱剂时,则能分别将dCMP、dAMP、TMP、dGMP完全分离.

Separating and processing technique of 5..- Deoxymononucleotides from fish spermary of chub mackerel

The process of digesting DNA - Na obtained from f ish spermary of chub mackerel into 5..- Deoxymononucleotides by using 5..- phosphodiesterase f rom Penicillium citrinum, M71 was studied. The 201 .. 8 anion exchange resin was used in the separation. The conditions for setting samples are height of column bed 105mm, diameter of column bed 45mm, sample concentration 213mg..mL- 1 and eluting flow..rate 0. 5mL..cm- 2 ..min- 1. The results of the separation indicated 5..- deoxymononucleotides components could be fully eluted as a whole peak by the elut ing agent, 0. 005 M HCl and 0. 04M NaCl. And the use of a few modified eluting agent s, i. e. 0. 001 8M HCl, 0. 002 8M HCl, 0. 036M NaCl( pH6. 0) and 0. 005M HCl+ 0. 02M NaCl could bring about perfect and respective elution of dCMP, dAMP, TMP and dGMP.