2 × Taq Platinum PCR Umxube

I-Ultra-emsulwa ye-HotStart ukuthembeka okuphezulu kwi-DNA polymerase.

I-Taq Platinum DNA Polymerase yicomputer eguqulweyo yeHotStart Taq polymerase enomsebenzi we-3'-5 'woxolelo kunye nomsebenzi we-5'-3' woxolelo. Umsebenzi we-enzyme weTaq Platinum DNA Polymerase ivaliwe kubushushu begumbi. Umsebenzi wayo unokusebenza kuphela emva kokufudumeza kwi-94 ° C kangange-5-10 min, oko ke kuthintele ukukhulisa okungangqinelaniyo okubangelwa kukuncitshiswa okungafunekiyo okanye i-primer dimer kubushushu obuphantsi ngaphambi komjikelo wokuqala wokuphendula kwe-PCR, kunye nokuphucula kakhulu uvakalelo kunye nokucaciswa kwempendulo ye-PCR. Ukongeza, i-Taq Platinum DNA Polymerase inokunyaniseka okuphezulu, okuyeyona nto yesibini ilungileyo kwi-Pfu polymerase. Isantya sokongezwa kwe-DNA polymerization ikhawuleza kunePfu polymerase kwaye ukusebenza kokunyusa kuphezulu.

Ikati. Hayi Ubungakanani bokuPakisha
4992789 5x1ml
4992790 5 × 1 ml

Iinkcukacha Product

Umzekelo wovavanyo

FAQ

Iimpawu zemveliso

Ingcaciso yomsebenzi

Iyunithi e-1 (U) Taq Platinum DNA Polymerase Umsebenzi uchazwa njengesixa se-enzyme efunekayo ukufaka i-10 nmol deoxynucleotides kwizinto ezingenakunyibilika kwi-asidi kwi-74 ° C ngaphakathi kwe-30 min usebenzisa i-salmon sperm DNA esebenzayo njengetemplate / primer.

Ulawulo lwemeko

Ukucoceka nge-SDS-PAGE ukubonwa kungaphezulu kwe-99%; Akukho msebenzi we-nuclease wangaphandle ufunyenwe; Ikopi enye yemfuza kwimfuzo yabantu inokukhulisa ngokufanelekileyo; Akukho lutshintsho lubalulekileyo lomsebenzi xa lugcinwe kubushushu begumbi iveki enye.

Iiparamitha zoBugcisa eziPhambili

Inomsebenzi wokuxolelwa u-5'-3 'kunye nomsebenzi we-3'-5' wokuxolelwa, kwaye ukuthembeka kwayo kukufutshane nePfu polymerase. Isantya sokongezwa kweTaq Platinum Polymerase sikhawuleza kunePfu polymerase kwaye ukusebenza kokunyusa kuphezulu. Iimveliso zePCR zinokuhanjiswa ngokuthe ngqo kwisiphelo esingacacanga okanye senziwe nge vector ye TA. Ukuba ukusebenza kobumbano kufuneka kuphuculwe, kuyacetyiswa ukuba kuhlanjululwe kuqala kwaye kongezwe ii-3'-dA overhangs ngaphambi kokuhlangana kwi-vector ye-TA.

Ityhubhu enye yeTaq Platinum MasterMix (isiQinisekiso seMveliso ePhakamileyo seTekhnoloji)

■ I-Taq Platinum MasterMix iphucule imeko ethile kunye nobuntununtunu bokuphendula kwe-PCR kwaye inokwandisa iitemplate ezimbaxa ezinomxholo ophezulu we-GC, ubume besekondari nokunye okunjalo. Ezisezantsi njengeekopi ezi-2 zetemplate ekujoliswe kuyo zinokwandiswa, kuqinisekiswe iziphumo zovavanyo ezichanekileyo ngakumbi.

■ Ifomula eyodwa ye-Taq Platinum MasterMix yenza ukuba inkqubo yokuphendula izinzile, kwaye umsebenzi awuyi kuchaphazeleka ngumkhenkce ophindaphindiweyo okanye ukugcinwa kwexesha elide kwi-4 ° C.

■ Isisombululo esixubileyo nesilungisiweyo esenziwe kwangaphambili se-PCR singenza umsebenzi ukhawuleze kwaye ube lula, ukunciphisa kakhulu uxinzelelo lwabasebenzi kunye nempazamo yokulinganisa. Ukusebenza okuphezulu kwe-PCR kunye ne-optimizer nayo ifakiwe kumxube, ocutha iimfuno kwiimeko ze-PCR.

This Le mveliso ineenkqubo ezinedayi kunye nezo zingenadayi. Imveliso yedayi ene-MasterMix yedayi inokuchongwa ngokuthe ngqo emva kwePCR, ngaphandle kokongeza ukulayishwa kwesikhuseli.

Izicelo

Inokuthi ithathe indawo yePfu polymerase yokwandisa iimveliso eziphezulu zokunyaniseka ezivela kwiitemplate ezintsonkothileyo ezinje ngee-genomes, kwaye kufanelekile kwizicelo ezinje ngokubumba izakhi zofuzo, ukuguqulwa kwendawo ethile kunye nohlalutyo lwe-nucleotide polymorphism (SNP), njl.

Amanyathelo okhuseleko kuyilo lwe-PCR Primers:

Ubude bokuqala buhlala bu-20-25 mer. Nangona kunjalo, xa usenza isiqwenga sePCR eside, ubude bokuqala bonyuswe buye kwi-30-35 mer.

■ Akukho kudityaniswa kokudibanisa phakathi kwezi zimbini zokuqala, ngakumbi kwiziseko ezi-3 zokugqibela esiphelweni sesi-3.

■ Umxholo we-GC kufuneka ube yi-50-60%, kwaye uthintele i-GC okanye i-AT. Ukwenza i-primer kunye netemplate zibambe ngxi, thintela ulwakhiwo lwe-AT kwisiphelo se-3.

■ Kuphephe ukuqala ngokwenza ulwakhiwo lwesibini.

■ Khetha ii-primers ezimbini ezinamaqondo obushushu e-Tm asondeleleneyo.

Ukubalwa kwexabiso le-Tm lee-Primers ze-PCR:

■ Xa i-primer ingaphantsi kwama-20 mer: Tm = 2 ° C × (A + T) + 4 ° C × (G + C).

■ Xa i-primer ingaphezulu kwe-20 mer: Tm = 81.5 + 0.41 × (GC%) - 600 / L, apho L ubude be-primer.

■ Cwangcisa ubushushu obongelayo (Tm-5) ° C.

Igalelo lePCR Primer

Ukufakwa kokugqibela koxinzelelo lwee-primers kunokukhethwa phakathi kwe-0.1 μM kunye ne-1.0 μM. Ukuphantsi kakhulu koxinzelelo lwe-primer kukhokelela kwisivuno esisezantsi seemveliso zokukhulisa, ngelixa ukuphakama kakhulu koxinzelelo lwe-primer kuthambekele ngakumbi ekukhuliseni okungachazwanga. Ngokwesiqhelo, xa inani le-template ye-DNA inkulu okanye inzima itemplate ye-DNA (enjenge-DNA yomntu) isetyenziswa njengetemplate, uxinzelelo lwe-primer kufuneka lube sezantsi. Xa inani leetemplate le-DNA lincinci okanye lilula itemplate ye-DNA (umzekelo, iplasmid DNA, njl. Njl.

Zonke iimveliso zingenziwa ngokwezifiso kwi-ODM / OEM. Iinkcukacha,nceda ucofe iNkonzo eChongiweyo (i-ODM / i-OEM)


  • Egqithileyo
  • Okulandelayo:

  • product_certificate04 product_certificate01 product_certificate03 product_certificate02
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    Experimental ExampleExperimental Example Sebenzisa i-genomic DNA njengetemplate yokwandisa isiqwenga se-1 kb. Emva kokuphendula kwe-PCR, thatha i-5 μl yokufumanisa i-electrophoresis.
    Q: Akukho zixhobo zokukhulisa

    Itemplate ye-A-1

    ■ Itemplate iqulethe ukungcola kweprotein okanye i-Taq inhibitors, njl njl. —Purify ithemplate ye-DNA, susa ukungcola kweprotein okanye ukhuphe i-DNA yeseti kunye neekiti zokucoca.

    ■ Ukuchazwa kweetemplate akuphelelanga ——Ukunyusa ngokufanelekileyo ubushushu bexesha kunye nokwandisa ixesha lokwenza oko.

    ■ Ukuhla komgangatho wetemplate- Lungisa kwakhona itemplate.

    I-A-2 Primer

    ■ Umgangatho ophantsi wee-primers -—Re-synthesize the primer.

    ■ ukuthotywa kwePrimer——Faka iziqwengana eziphezulu zoxinaniso zibe ngumthamo omncinci wolondolozo. Kunqande ukukhenkceza okuninzi kunye nokunyibilika okanye ixesha elide i-4 ° C ikhutshiwe.

    ■ Uyilo olungafanelekanga lwezinto zokuqala (umz.

    I-A-3 Mg2+Uxinzelelo

    ■ Mg2+ uxinzelelo luphantsi kakhulu ——Ukunyusa ngokufanelekileyo uMg2+ Uxinzelelo: Lungiselela iMg2+ uxinzelelo ngothotho lwempendulo ukusuka kwi-1 mM ukuya kwi-3 mM ngexeshana le-0.5 mM ukumisela eyona Mg2+ Uxinzelelo lwetemplate nganye kunye ne-primer.

    Ubushushu be-A-4 bokuTshintsha

    The Amaqondo obushushu aphezulu afakela umbane achaphazela ukubopha kwento yokuqala kunye netemplate. —Ukunciphisa ubushushu obongezelelekileyo kwaye wandise imeko ngegradient eyi-2 ° C.

    Ixesha le-5 lokongezwa

    ■ Ixesha elifutshane lokwandiswa- Yandisa ixesha lolwandiso.

    Umbuzo: Ubuxoki

    Phenomena: Iisampulu ezingathandekiyo zikwabonisa ukulandelelana kwebhendi.

    Ungcoliseko lwe-A-1 lwe-PCR

    ■ Ungcoliseko lomnqamlezo wolandelelwano ekujoliswe kulo okanye iimveliso zokukhulisa ——Ukunyamekela ukungahambi ngesampulu yesampulu enolandelelwano ekujoliswe kulo kwisampulu engeyiyo okanye uchithe ityhubhu yecentrifuge. Izinto ezenziwayo okanye izixhobo kufuneka zenziwe ngokuzenzekelayo ukuze kupheliswe iicicic acid ezikhoyo, kwaye ubukho bengcoliseko kufuneka bugqitywe ngovavanyo olubi lokulawula.

    ■ Ungcoliseko olungenanjongo —Faka iizincedisi uze uzigcine kubushushu obuphantsi.

    Inkulumbuso ye-A-2r

    ■ Mg2+ uxinzelelo luphantsi kakhulu ——Ukunyusa ngokufanelekileyo uMg2+ Uxinzelelo: Lungiselela iMg2+ uxinzelelo ngothotho lwempendulo ukusuka kwi-1 mM ukuya kwi-3 mM ngexeshana le-0.5 mM ukumisela eyona Mg2+ Uxinzelelo lwetemplate nganye kunye ne-primer.

    ■ Uyilo olungafanelekanga lokuqala, kwaye ulandelelwano ekujoliswe kulo lunehomeology ngolandelelwano olungajoliswanga. -Ukuyila ngokutsha ii-primers.

    Q: Ukwandiswa okungachazwanga

    I-Phenomena: Iibhendi zokunyusa i-PCR azihambelani nobungakanani obulindelweyo, nokuba bukhulu okanye bincinci, okanye ngamanye amaxesha zombini izibophelelo ezithile kunye neebhendi zokunyusa ezingachazwanga.

    I-A-1 Primer

    ■ Ukuchaneka kokukodwa kokuqala

    -Ukuyila ngokutsha.

    ■ Uxinzelelo lwe-primer luphezulu kakhulu — -Ukunyusa ngokufanelekileyo ubushushu be-denaturation kunye nokwandisa ixesha le-denaturation.

    I-A-2 Mg2+ Uxinzelelo

    ■ UMg2+ Ukugxininisa kuphezulu kakhulu — -Ukunciphisa ngokufanelekileyo i-Mg2 + yoxinaniso: Sebenzisa i-Mg2+ uxinzelelo ngothotho lwempendulo ukusuka kwi-1 mM ukuya kwi-3 mM ngexeshana le-0.5 mM ukumisela eyona Mg2+ Uxinzelelo lwetemplate nganye kunye ne-primer.

    A-3 Polymerase enokunyangeka

    ■ Isixa se-enzyme esigqithisileyo —— Nciphisa isixa se-enzyme ngokufanelekileyo kumakhefu e-0.5 U.

    Ubushushu be-A-4 bokuTshintsha

    ■ Iqondo lobushushu lokufakelwa liphantsi kakhulu ——Ukunyusa ngokufanelekileyo ubushushu obongezwe okanye sebenzisa indlela yokubamba enezigaba ezibini

    Imijikelezo ye-A-5 ye-PCR

    ■ Imijikelo ye-PCR emininzi kakhulu —— Nciphisa inani lemijikelezo ye-PCR.

    Q: Iipatchy okanye i-smear band

    I-A-1 PrimerUkucaciswa kokubi -Yila kwakhona i-primer, tshintsha indawo kunye nobude be-primer ukongeza ukungangqinelani kwayo; okanye wenze i-PCR enendawo yokuhlala.

    I-A-2 template yeDNA

    —Ithemplate ayihlambulukanga -Hlambulula itemplate okanye ukhuphe i-DNA eneekiti zokucoca.

    I-A-3 Mg2+ Uxinzelelo

    —Mg2+ ingxinano iphezulu kakhulu -—Ukunciphisa ngokufanelekileyo uMg2+ Uxinzelelo: Lungiselela iMg2+ uxinzelelo ngothotho lwempendulo ukusuka kwi-1 mM ukuya kwi-3 mM ngexeshana le-0.5 mM ukumisela eyona Mg2+ Uxinzelelo lwetemplate nganye kunye ne-primer.

    I-4-dNTP

    —— Uxinaniso lwe-dNTPs luphezulu kakhulu —— Nciphisa uxinaniso lwe-dNTP ngokufanelekileyo

    Ubushushu be-5-Annealing

    —— Amaqondo obushushu aphantsi athathelwa phantsi ——Ukunyusa ngokufanelekileyo iqondo lobushushu elihlanganisiweyo

    Imijikelo ye-A-6

    —Imijikelo emininzi ——Yandisa inani lomjikelo

    Q: Yimalini itemplate yeDNA ekufuneka ifakwe kwi-50 μl PCR reaction system?
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    Umbuzo: Ungawandisa njani amaqhekeza amade?

    Isinyathelo sokuqala kukukhetha i-polymerase efanelekileyo. Rhoqo Taq polymerase ayinakuphinda ifundwe ngenxa yokunqongophala kwemisebenzi ye-3'-5 'exonuclease, kwaye ukungangqinelani kuya kunciphisa kakhulu ukwandiswa kweziqwengana. Ke ngoko, i-Taq polymerase eqhelekileyo ayinako ukukhulisa ngokufanelekileyo iziqwengana ekujoliswe kuzo ezinkulu kune-5 kb. I-Taq polymerase enenguqulelo ekhethekileyo okanye enye i-high fidelity polymerase kufuneka ikhethwe ukuphucula ulwandiso kunye nokuhlangabezana neemfuno zokukhulisa iziqwengana ezinde. Ukongeza, ukukhula kwamaqhekeza amade kukwafuna uhlengahlengiso oluhambelanayo loyilo lokuqala, ixesha lokubonisa, ixesha lokwandiswa, i-pH yesixhobo, njl. Njl. Ukuthintela ukonakala kwetemplate, ixesha lokudlulisa kwi-94 ° C kufuneka licuthwe liye kwi-30 sec okanye ngaphantsi kumjikelo ngamnye, kwaye ixesha lokunyuka kobushushu liye kwi-94 ° C ngaphambi kokukhulisa kufuneka kube ngaphantsi komzuzu omnye. Ngapha koko, ukuseta ubushushu obandisiweyo malunga ne-68 ° C kunye nokuyila ixesha lolwandiso ngokwenqanaba le-1 kb / min kunokuqinisekisa ukukhulisa ngokufanelekileyo iziqwengana ezinde.

    Q: Ungakuphucula njani ukunyaniseka kokukhulisa i-PCR?

    Ixabiso lempazamo zokukhulisa i-PCR linokuncitshiswa ngokusebenzisa iipolymerase zeDNA ezahlukeneyo ngokuthembeka okuphezulu. Kuzo zonke i-Taq DNA polymerases ezifumanekayo ukuza kuthi ga ngoku, iPfu enzyme ineyona mpazamo iphantsi kunye nokunyaniseka okuphezulu (jonga itafile eqhotyoshelweyo). Ukongeza kukhetho lwe-enzyme, abaphandi banokuqhubeka nokunciphisa inqanaba lokutshintsha kwe-PCR ngokwandisa iimeko zokuphendula, kubandakanya nokwenza ukwakheka kwesixokelelwano, uxinzelelo lwe-polymerase enokunyanga kunye nokwenza nombolo yomjikelo wePCR.

    Bhala umyalezo wakho apha uze uyithumele kuthi