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ÎÒÕûÀíµÄPCR×ÊÁÏ.¹©´ó¼Ò·ÖÏí.

PCRʵÑé¼¼ÇÉ

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1. primeÀíÏëµÄ£¬Ö»Í¬Ä¿µÄÐòÁÐÁ½²àµÄµ¥Ò»ÐòÁжø·ÇÆäËûÐòÁÐÍË»ðµÄÒýÎïÒª·ûºÏÏÂÃæµÄ һЩÌõ¼þ
a. ×ã¹»³¤,18-24bp,ÒÔ±£Ö¤ÌØÒìÐÔ.µ±È»²»ÊÇ˵Խ³¤Ô½ºÃ,Ì«³¤µÄÒýÎïͬÑù»á½µµÍÌØÒìÐÔ,²¢ÇÒ½µµÍ²úÁ¿
b. GC% 40%~~~~60%
c. 5'¶ËºÍÖмäÐòÁÐÒª¶àGC,ÒÔÔö¼ÓÎȶ¨ÐÔ
d. ±ÜÃâ3'¶ËGC rich, ×îºó3¸öBASE²»ÒªÓÐGC,»òÕß×îºó5¸öÓÐ3¸ö²»ÒªÊÇGC
e. ±ÜÃâ3'¶ËµÄ»¥²¹, ·ñÔòÈÝÒ×Ôì³ÉDIMER
f. ±ÜÃâ3'¶ËµÄ´íÅä
g. ±ÜÃâÄÚ²¿Ðγɶþ¼¶½á¹¹
h. ¸½¼ÓÐòÁÐ(RT site, Promoter sequence)¼Óµ½5'¶Ë, ÔÚËãTmֵʱ²»Ëã,µ«ÔÚ¼ì²â»¥²¹ºÍ¶þ¼¶½á¹¹ÊÇÒª¼ÓÉÏËüÃÇ
i. ʹÓü沢ÒýÎïʱ, Òª²Î¿¼ÃÜÂë×ÓʹÓñí,×¢ÒâÉúÎïµÄÆ«ºÃÐÔ,²»ÒªÔÚ3'¶ËʹÓü沢ÒýÎï,²¢Ê¹Óà ½Ï¸ßµÄÒýÎïŨ¶È(1uM-3uM)
j. ×îºÃѧ»áʹÓÃÒ»ÖÖdesign software. PP5,Oligo6,DNAstar, Vector NTI, Online¡¡desgin et al.
* ÒýÎïµÄÁíÒ»¸öÖØÒª²ÎÊýÊÇÈÛ½âζȣ¨Tm£©¡£ÕâÊǵ±50£¥µÄÒýÎïºÍ»¥²¹ÐòÁбíÏÖΪ˫Á´DNA·Ö×ÓʱµÄζÈ.Tm¶ÔÓÚÉ趨PCRÍË»ðζÈÊDZØÐèµÄ¡£ÔÚÀíÏë״̬Ï£¬ÍË»ðζÈ×ã¹»µÍ£¬ÒÔ±£Ö¤ÒýÎïͬĿµÄÐòÁÐÓÐЧÍ˻𣬠ͬʱ»¹Òª×ã¹»¸ß£¬ÒÔ¼õÉÙ·ÇÌØÒìÐÔ½áºÏ¡£ºÏÀíµÄÍË»ðζȴÓ55¡æµ½70¡æ¡£ÍË»ðζÈÒ»°ãÉ趨±ÈÒýÎïµÄ TmµÍ5¡æ¡£
É趨TmÓм¸ÖÖ¹«Ê½¡£ÓеÄÊÇÀ´Ô´ÓÚ¸ßÑÎÈÜÒºÖеÄÔÓ½»£¬ÊÊÓÃÓÚСÓÚ18¼î»ùµÄÒýÎï¡£
ÓеÄÊǸù¾ÝGCº¬Á¿¹ÀËãTm¡£È·¶¨ÒýÎïTm×î¿ÉÐŵķ½·¨ÊǽüÁÚ·ÖÎö·¨¡£ÕâÖÖ·½·¨´ÓÐòÁÐÒ»¼¶½á¹¹ºÍ ÏàÁÚ¼î»ùµÄÌØÐÔÔ¤²âÒýÎïµÄÔÓ½»Îȶ¨ÐÔ¡£´ó²¿·Ö¼ÆËã»ú³ÌÐòʹÓýüÁÚ·ÖÎö·¨¡£
¸ù¾ÝËùʹÓõĹ«Ê½¼°ÒýÎïÐòÁеIJ»Í¬£¬Tm»á²îÒìºÜ´ó¡£ÒòΪ´ó²¿·Ö¹«Ê½Ìṩһ¸ö¹ÀËãµÄTmÖµ£¬ËùÓÐÍË»ðζÈÖ»ÊÇÒ»¸öÆðʼµã¡£¿ÉÒÔͨ¹ý·ÖÎö¼¸¸öÖð²½Ìá¸ßÍË»ðζȵķ´Ó¦ÒÔÌá¸ßÌØÒìÐÔ¡£¿ªÊ¼µÍÓÚ¹ÀËãµÄTm5¡æ£¬ÒÔ2¡æÎªÔöÁ¿£¬Öð²½Ìá¸ßÍË»ðζȡ£½Ï¸ßµÄÍË»ðζȻá¼õÉÙÒýÎï¶þ¾ÛÌåºÍ·ÇÌØÒìÐÔ²úÎïµÄÐγɡ£
Ϊ»ñµÃ×î¼Ñ½á¹û£¬Á½¸öÒýÎïÓ¦¾ßÓнüËÆµÄTmÖµ¡£ÒýÎï¶ÔµÄTm²îÒìÈç¹û³¬¹ý5¡æ£¬¾Í»áÒýÎïÔÚÑ­»·ÖÐʹÓýϵ͵ÄÍË»ðζȶø±íÏÖ³öÃ÷ÏԵĴíÎóÆðʼ¡£Èç¹ûÁ½¸öÒýÎïTm²»Í¬£¬½«ÍË»ðζÈÉ趨Ϊ±È×îµÍµÄTmµÍ5¡æ
»òÕßΪÁËÌá¸ßÌØÒìÐÔ£¬¿ÉÒÔÔÚ¸ù¾Ý½Ï¸ßTmÉè¼ÆµÄÍË»ðζÈÏȽøÐÐ5¸öÑ­»·£¬È»ºóÔÚ¸ù¾Ý½ÏµÍTmÉè¼ÆµÄÍË»ðζȽøÐÐÊ£ÓàµÄÑ­»·¡£ÕâʹµÃÔÚ½ÏΪÑϽôµÄÌõ¼þÏ¿ÉÒÔ»ñµÃÄ¿µÄÄ£°åµÄ²¿·Ö¿½±´¡£
2. stability of primers
¶¨ÖÆÒýÎïµÄ±ê×¼´¿¶È¶ÔÓÚ´ó¶àÊýPCRÓ¦ÓÃÊÇ×ã¹»µÄ¡£
ÒýÎï²úÁ¿Êܺϳɻ¯Ñ§µÄЧÂʼ°´¿»¯·½·¨µÄÓ°Ïì¡£¶¨ÖÆÒýÎïÒԸɷÛÐÎʽÔËÊä¡£×îºÃÔÚTEÖØÈÜÒýÎʹÆä×îÖÕŨ¶ÈΪ100¦ÌM¡£TE±ÈÈ¥Àë×ÓË®ºÃ£¬ÒòΪˮµÄpH¾­³£Æ«Ëᣬ»áÒýÆð¹ÑºËÜÕµÄË®½â¡£ ÒýÎïµÄÎȶ¨ÐÔÒÀÀµÓÚ´¢´æÌõ¼þ¡£Ó¦½«¸É·ÛºÍÈܽâµÄÒýÎï´¢´æÔÚ-20¡æ¡£ÒÔ´óÓÚ10¦ÌMŨ¶ÈÈÜÓÚTEµÄÒýÎïÔÚ -20¡æ¿ÉÒÔÎȶ¨±£´æ6¸öÔ£¬µ«ÔÚÊÒΣ¨15¡æµ½30¡æ£©½öÄܱ£´æ²»µ½1ÖÜ¡£¸É·ÛÒýÎï¿ÉÒÔÔÚ-20¡æ±£´æÖÁÉÙ1Ä꣬ÔÚÊÒΣ¨15¡æµ½30¡æ£©×î¶à¿ÉÒÔ±£´æ2¸öÔ¡£

3. optimize reactants concentration
a. magnesiom ions
Mg2+Àë×ÓµÄ×÷ÓÃÖ÷ÒªÊÇ dNTP-Mg ÓëºËËá¹Ç¼ÜÏ໥×÷Óà ²¢ÄÜÓ°ÏìPolymeraseµÄ»îÐÔ£¬Ò»°ãµÄÇé¿öÏ Mg2+µÄŨ¶ÈÔÚ0.5-5mMÖ®¼äµ÷Õû£¬Í¬ÑùÒª¼ÇסµÄÊÇÔÚµ÷ÕûÁËdNTPsµÄŨ¶ÈºóÒªÏàÓ¦µÄµ÷ÕûMg2+Àë×ÓµÄŨ¶È£¬¶Ôʵʱ¶¨Á¿PCR£¬Ê¹ÓÃ3µ½5mM´øÓÐÓ«¹â̽ÕëµÄþÀë×ÓÈÜÒº
b. ÆäËûµÄÀë×Ó
NH4+ K+¶¼»áÓ°ÏìPCR£¬Ôö¼ÓK+µÄŨ¶Èºó, »áÒòΪÖкÍÁ˺ËËá¹Ç¼ÜÉÏÁ×Ëá»ùÍŵĸºµçºÉ¶øÓ°ÏìÍË»ðµÄζÈ,´Ó¶ø½µµÍÁËPCRµÄ ÑϽ÷ÐÔ(stringency)£¬NH4+Ò²ÓÐÏàͬµÄ×÷ÓÃ.µ±È», ¹ý¸ßµÄÑôÀë×ÓŨ¶È(KCL>0.2M)ʱ, DNAÔÚ940C¸ù±¾²»»á·¢Éú±äÐÔ, µ±È»Ò²¾ÍÎÞ´Ó̸ÆðPCRÁË.
c. polymerase
²»Í¬¹«Ë¾µÄøЧÓÐËù²»Í¬,ÐèÒªoperator×Ô¼ºÕÆÎÕÊʺϵÄøµÄŨ¶È£¬Ò»Ð©¸ß±£ÕæÃ»µÄЧÂÊÒªÔ¶Ô¶µÍÓÚTaq polymerase,ËùÒÔ¿ÉÄÜÐèÒªµÄøµÄÁ¿Ò²Òª´óһЩ. ÁíÍâ, Ò»°ãµÄ Çé¿öÏÂ, ±äÐÔµÄζȿÉÒÔʹÓÃ90~920C, ±äÐÔµÄʱ¼äÒ²¿ÉÒÔËõ¶Ì,´Ó¶ø±£Ö¤polymeraseµÄ»îÐÔ
d. template
50ul PCR SYSTEM
human g DNA 0.1ug-1ug
E.Coli 10ng-100ng
Lamada DNA 0.5ng-5ng
Plasmid DNA 0.1ng-10ng
4. termperature
a. denaturation
³£¹æÊÇ940C 5·ÖÖÓ, GC RichµÄÃþ°åÊÇ950C 5·ÖÖÓ
³ýÁËGC RichÍâ, ³£¹æµÄAPPLICATIONS¿ÉÒÔ½«Õⲿ·Öʱ¼äËõ¶Ìµ½1µ½2·ÖÖÓ, »òÕßÔÚCYCLE 1ʱ¸øÓè½Ï³¤µÄʱ¼ä,¶øÈ¡Ïû¿ªÊ¼µÄdenaturation
b. annealing
ÖØµãµ½ÁË£ºÒ»°ãÇé¿öÏÂ, ÊÇ´Ó55¶È¿ªÊ¼.¸ù¾ÝÇé¿öÅäºÏÒÔMgÀë×ÓŨ¶È½øÐе÷Õû. ÓÐÌõ¼þµÄ¿ÉÒÔ×ögradient PCR. ÍË»ðµÄʱ¼äÔÚ30-60S, ʱ¼ä¶ÌһЩ¿ÉÒԵõ½¸üºÃµÄЧ¹û. ÒòΪ, polymerase ÔÚ annealing temp.ʱҲ»áÓÐһЩ»îÐÔ. ËùÒÔÔÚA.T.µÄʱ¼ä¹ý³¤, »á¼«´óµÄÔö¼Ó·ÇÌØÒìÐÔÀ©ÔöµÄ·çÏÕ£¬ÁíÍâ,ÔÚ¶ÔÓÚһЩÀ§ÄÑ»§, ±ÈÈç´ÓgDNAÀïÀ©Ôö´óƬ¶Î, »¹¿ÉʹÓÃtwo step PCR.
5. touchdown PCR
Ô­ÀíºÜ¼òµ¥,µ«µÄÈ·ÊÇÒ»¸öºÜÓÐÓõķ½·¨¡£¾Ù¸öÀý×Ó£¬ANNEALING TEMP. 55¶È
940C 5min 940C 30s 600C 30s 720C 1min 2cycles 940C 30s 590C 30s
720C 1min 2cycles 940C 30s 580C 30s 720C 1min 2cycles 940C 30s
510C 30s 720C 1min 2cycles 940C 30s 500C 30s
720C 1min 20cycles 720C 5min
6. hot start PCR
ÈÈÆô¶¯PCRÊdzýÁ˺õÄÒýÎïÉè¼ÆÖ®Í⣬Ìá¸ßPCRÌØÒìÐÔ×îÖØÒªµÄ·½·¨Ö®Ò»¡£¾¡¹ÜTaq DNA¾ÛºÏøµÄ×î¼ÑÑÓÉìζÈÔÚ72¡æ£¬¾ÛºÏøÔÚÊÒÎÂÈÔÈ»ÓлîÐÔ¡£Òò´Ë£¬ÔÚ½øÐÐPCR·´Ó¦ÅäÖÆ¹ý³ÌÖУ¬ÒÔ¼°ÔÚÈÈÑ­»·¸Õ¿ªÊ¼£¬±£ÎÂζȵÍÓÚÍË»ðζÈʱ»á²úÉú·ÇÌØÒìÐԵIJúÎï¡£ÕâЩ·ÇÌØÒìÐÔ²úÎïÒ»µ©Ðγɣ¬¾Í»á±»ÓÐЧÀ©Ôö¡£ÔÚÓÃÓÚÒýÎïÉè¼ÆµÄλµãÒòΪÒÅ´«Ôª¼þµÄ¶¨Î»¶øÊÜÏÞʱ£¬Èçsite-directedÍ»±ä¡¢±í´ï¿Ë¡»òÓÃÓÚDNA¹¤³ÌµÄÒÅ´«Ôª¼þµÄ¹¹½¨ºÍ²Ù×÷£¬ÈÈÆô¶¯PCRÓÈΪÓÐЧ¡£
ÏÞÖÆTaq DNA¾ÛºÏø»îÐԵij£Ó÷½·¨ÊÇÔÚ±ùÉÏÅäÖÆPCR·´Ó¦Òº£¬²¢½«ÆäÖÃÓÚÔ¤ÈȵÄPCRÒÇ¡£ÕâÖÖ·½·¨ ¼òµ¥±ãÒË£¬µ«²¢²»ÄÜÍê³ÉÒÖÖÆÃ¸µÄ»îÐÔ£¬Òò´Ë²¢²»ÄÜÍêÈ«Ïû³ý·ÇÌØÒìÐÔ²úÎïµÄÀ©Ôö¡£
ÈÈÆô¶¯Í¨¹ýÒÖÖÆÒ»ÖÖ»ù±¾³É·ÖÑÓ³ÙDNAºÏ³É£¬Ö±µ½PCRÒÇ´ïµ½±äÐÔζȡ£°üÀ¨ÑÓ»º¼ÓÈëTaq DNA¾ÛºÏ ø£¬ÔÚ·´Ó¦Ìåϵ´ïµ½90¶Èʱ£¬PAUSE£¬½«Î¶ȱ£³ÖÔÚ70¶ÈÒÔÉÏ£¬ÊÖ¹¤¼ÓÈëpolymerase£¬µ«Õâ¸ö·½·¨¹ýÓÚ·³Ëö£¬ ÓÈÆäÊǶԸßͨÁ¿Ó¦Ó㬲¢ÈÝÒ×Ôì³ÉÎÛȾ¡£ÆäËûµÄÈÈÆô¶¯·½·¨Ê¹ÓÃÀ¯·À»¤²ã½«Ò»ÖÖ»ù±¾ ³É·Ö£¬ÈëþÀë×Ó»òø£¬°ü¹üÆðÀ´£¬»òÕß½«·´Ó¦³É·Ö£¬ÈçÄ£°åºÍ»º³åÒº£¬ÎïÀíµØ¸ôÀ뿪¡£
7. Booster PCR
ÎÒÃÇÖªµÀ1ug human genomic DNA ´óÔ¼ÔÚ3X105¸öÄ£°å·Ö×Ó,ÕâÑùµÄÄ£°å·Ö×ÓÊýÄ¿¿ÉÒÔÊÇÒýÎïÓëÄ£°åºÜºÃµÄ½áºÏ. µ±Ä£°åµÄŨ¶È¹ýµÍ,±ÈÈçµÍÓÚ100¸ö·Ö×Óʱ, ÒýÎïºÍÄ£°åÖ®¼ä¾ÍºÜÄÑ·¢Éú·´Ó¦. ÒýÎïÈÝÒ××ÔÉí½øÐз´Ó¦Ðγɶþ¾ÛÌå.ÕâÑù¾ÍÓÐÀ´Á˸ö booster PCR ÎÒÒ»Ö±ÕÒ²»µ½ºÏÊʵĴÊÀ´·­ÒëÕâ¸öbooster.
¾ßÌåÊÇÕâÑùµÄ.¿ªÊ¼¼¸¸öcycles±£³ÖprimerµÄµÍŨ¶È,±£Ö¤primer:templateµÄmolar ratioÔÚ10 7~ 10 8. ÒÔÈ·±£¿ªÊ¼À©ÔöµÄ׼ȷÐÔ.È»ºóbooste PrimerµÄŨ¶Èµ½Õý³£µÄˮƽ
8. Ñ­»·ÊýºÍ³¤¶È
È·¶¨Ñ­»·ÊýµÄ»ù±¾Ô­ÀíÊÇ: ²úÎïÄܹ»±£Ö¤Äã½øÒ»²½·ÖÎö²Ù×÷µÄ×îСѭ»·Êý.ÒòΪ¹ý¶àµÄÑ­»·ÊýÈÝÒ×Ôì ³ÉERRORSºÍ·ÇÌØÒìÐÔ²úÎïµÄ»ýÀÛ ²úÎïµÄÁ¿²»¹», ÓÅ»¯µÄ·½·¨ÓÐ:
1. Ôö¼ÓTEMPLATE
2. Ôö¼ÓÑ­»·Êý
ÈçºÎÈ·¶¨Ñ­»·Êý,ÓÐÒ»¸ö·½·¨.
×öÒ»¸öPCRÌåϵ,40Ñ­»·,50ul, ·Ö±ðÔÚ20,25,30,35Ñ­»·Ê±´ÓÌåϵÖÐÈ¡5ul,Ò»ÆðÅܵçÓ¾·ÖÎö.´Ó¶øÈ·¶¨×î¼ÑµÄÑ­»·Êý
ÁíÒ»¸ö»áÓ°ÏìPCRÌØÒìÐÔµÄÊÇPCR cyclingʱÔÚÁ½¸öζȼä±ä»¯µÄËÙÂÊ(ramping rate).µ±È»ÊÇÔ½¸ß Ô½ºÃ.²»¹ýÔÛÃǴ󲿷ÖÌõ¼þÓÐÏÞ,¾ÍÄÇô¼¸Ì¨PCRÒÇ,ҲûÓжàÉÙÌôÑ¡µÄÓàµØ
9. thermal cycler
PCRÒǵÄÒòËØÎÒÃǾ­³£ÈÝÒ׺öÊÓ.³¤Ê±¼äµÄʹÓúóÐèÒªµ÷ÕûPCRÒÇ,ÒÔ±£Ö¤ÆäÄܹ»µ½´ïÕýÈ·µÄζÈ.ÏÖÔÚµÄPCRÒÇ»ù±¾É϶¼ÓÐ×Լ칦ÄÜ(self-diagnosis).
10. PCR additives
¸½¼ÓÎï»òÕß˵enhancerʵÔÚÊǶàÖÖ¶àÑù. »ù±¾ÉϰüÀ¨¼¸Àà, Äܹ»Ôö¼Ó·´Ó¦ÍË»ðЧÂʵĻ¯Ñ§Òò×Ó, DNA½áºÏµ°°×ºÍһЩÉÌÒµÊÔ¼Á. »ù±¾µÄÔ­Àí²»ÍâÊÇÔö¼ÓÒýÎïÍË»ðÌØÒìÐÔ,¼õÉÙ´íÅä, Ôö¼Ó²úÎïµÄ³¤¶ÈºÍ²úÁ¿.
ÔÚGC RichÇé¿öÖÐ, additive¿ÉÒÔÔì³ÉÅä¶Ô¼î»ù¼äµÄµÄ²»Îȶ¨,´Ó¶øÌá¸ßÀ©ÔöµÄЧÂÊ.¶øÔÚÁíÒ»ÖÖÇé¿öÏÂ,additiveÓÉÓÚÔì³É´íÅäµÄprimer-template¸´ºÏÎïµÄ¼«´óµÄ²»Îȶ¨, ¶øÌá¸ßÁËÀ©ÔöµÄÖÒʵÐÔ.ҪעÒâµÄÊÇ,ûÓÐÍòÄܵÄenhancerÈ«²¿Í¨ÓÃ,ÐèÒªÄã¸ù¾Ý×Ô¼ºµÄÇé¿ö,×îºÃ½áºÏgradient pcrÑ¡Ôñ×îÓÅÌõ¼þ.
dimethyl sulfoxide(DMSO) up to 10%
formamide at 5%
trimethylammonium chloride 10-100uM
detergents such as Tween 20 0.1-2.5%
polyethylene glycol (PEG)6000 5-15%
glycerol 10-15%
single stranded DNA binding proteins
Gene 32 protein 1nM
E.coli single-stranded DNA binding protein 5uM
7 deaza-dGTP(for GC rich) 150uM with 50uM dGTP
ҪעÒâµÄÊÇ,DMSO,GLYCEROLµÈ»áÒÖÖÆpolymeraseµÄ»îÐÔ,ËùÒÔÐèÒªscouting³ö×îÊʵÄŨ¶È
11. Template DNA preparation
ÌáÈ¡DNAʱµÄÊÔ¼Á»áÒÖÖÆPCR·´Ó¦µÄ˳Àû½øÐÐ.Òò´ËÐèÒª¶ÔTEMPLATE DNA½øÐд¿»¯.ÌØ±ðÊÇSDS(<0.01%) µÄÇé¿öϾÍÄÜÇ¿ÁÒÒÖÖÆPCRµÄ½øÐÐ. ¿ÉÒÔ¼ÓÈëһЩnonionicÊÔ¼Á,ÈçTween, Nonid, TritionÖ®ÀàµÄ·´¹ýÀ´ÒÖÖÆSDS. »¹ÓÐproteinase KÒ²Òª³ý¸É¾», ²»È»»á½µ½âpolymerase.
12. Nested PCR
¼òµ¥µã˵ Éè¼ÆÁ½¶ÔÒýÎï, Ò»¶ÔÊdz¤µÄ, Ò»¶ÔÊǰüº¬ÔÚ³¤ÒýÎïÄÚµÄ, Óó¤ÒýÎïÀ©ÔöµÄ²úÎï×÷ΪµÚ¶þ´ÎÀ©ÔöµÄÄ£°å,ÕâÑù¿ÉÒÔÔö¼Ó²úÎïµÄÁ¿. ¶øÇÒ¿ÉÒÔ¼õÉÙ·ÇÌØÒìÐÔ´øºÍ´íÅäµÄÇé¿ö.
¸ß±£ÕæÃ¸
¸ßÎÂDNA POLYMERASEÊÇÒÔµ¥Á´DNA»òRNAΪģ°å£¬ÔÚdNTPºÍһЩÑôÀë×ӵĴæÔÚÇé¿öÏ£¬ÔÚÌØ¶¨µÄÒýÎïÖ¸µ¼Ï°´3'-5'·½ÏòºÏ³ÉDNA.°üÀ¨3ÖÖÀàÐÍ
a.5'-3'·½ÏòµÄDNAºÏ³ÉÄÜÁ¦,ûÓÐ3'-5'·½ÏòµÄÍâÇÐÃ¸ÌØÐÔ.ÈçTaq¼°ÆäÍ»±äÌå.ÕâÀàøµÄºÏ³ÉÄÜÁ¦Ç¿,ÒòΪËû²»¾ÀÕýºÏ³ÉÖгöÏÖµÄÍ»±ä
b.ÓëaÀàËÆ,ÓкϳɻîÐÔ,ûÓÐ3-5µÄÍâÇлîÐÔ.µ«ËûÃÇÄÜÒÔRNAΪģ°å,ºÏ³ÉDNA. ÈçTth DNA Polymerase
c.ÓÐDNA¾ÛºÏ»îÐÔ,ûÓÐÄæ×ªÂ¼»îÐÔ,µ«ÓÐ3-5·½ÏòµÄÍâÇÐø»îÐÔ.Èçpfu DNA Polymerase.¿ÉÒÔÌá¸ßÖÒʵÐÔ¡£µ«ÊÇÕâЩ¾ÛºÏøµÄ²úÁ¿±ÈTaq DNA¾ÛºÏøµÍ¡£
øµÄ»ìºÏÎï
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