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Ihe atụ nke HS Taq DNA Polymerase

Onyonyo egosipụtara HS Taq DNA Polymerase Foreasy
  • Ihe atụ nke HS Taq DNA Polymerase

Nkọwa ngwa:

Nkọwa dị elu: Enzyme nwere ọrụ mmalite na-ekpo ọkụ dị elu.

Nkwalite ngwa ngwa: 10 sk/kb.

Elu template adaptability: enwere ike iji mee ka ọ dị elu nke ọmaGCurunaụdị DNA dị iche iche siri ike ịkwalite.

Ikwesị ntụkwasị obi siri ike: Ikwesị ntụkwasị obi bụ ugboro 6of nkịtị Taq Enzyme.

ike foregene


Nkọwa ngwaahịa

Mkpado ngwaahịa

FAQ

Nkọwa

Foreasy HS Taq DNA Polymerase bụ enzyme Taq ọhụrụ egosipụtara na nje bacteria Escherichia coli engineering site na teknụzụ recombination gene.Mgbe a na-emeso enzyme ahụ na usoro pụrụ iche, ọ'A na-egbochi ọrụ s tupu ịgbalite ọkụ, si otú a na-egbochi mmụba na-abụghị nke a na-eme ka ọ bụrụ nke na-adịghị akọwapụta nke primers ma ọ bụ primer dimers n'okpuru ọnọdụ okpomọkụ dị ala.Ngwaahịa a dabara adaba maka PCR React nke ukwuuion, M ultiple x PCR, ọdịnaya GC dị elu (> 60%),ya nausoro nke abụọma ọ bụ ọzọike ndabere genomicsmmụba na nnukwu genomicsnchọpụta mmụba.Enzyme ahụ nwere ọrụ 5' 3' DNA polymerase na 5' → 3' ọrụ exonuclease, mana ọ nweghị ọrụ 3' → 5' exonuclease.

Ngwa ngwa

Akụkụ IM-01021 IM-01022 IM-01023
HS Taq DNA Polymerase (5 U/μL)  5000 U (1 ml)  50 KU (10 ml)  500 KU (100 ml)
2× Taq Reaction Buffer  25ml × 5  250 ml × 5  500 ml × 25

Atụmatụ & uru

- Nkọwa dị elu: enzyme nwere ọrụ mmalite dị elu.

- Mmụba ngwa ngwa: 10 sk/kb.

- Mgbanwe template dị elu: enwere ike iji mee ka elu dị elu rụọ ọrụ nke ọmaGCurunaụdị DNA dị iche iche siri ike ịkwalite.

- Ikwesị ntụkwasị obi siri ike: Ikwesị ntụkwasị obi bụ ugboro 6of nkịtị Taq Enzyme.

Ngwa ngwa

- PCR / qPCR dị iche iche na sistemụ PCR ozugbo

- Iberibe DNA agbakwunyere PCR

- DNA akara

- Usoro DNA

- PCR gbakwunyere A ọdụ

Nkọwa ihe omume

1U: Ọnụ ego nke enzyme achọrọ iji tinye 10 nmol nkeDNAn'ime ihe na-adịghị edozi acid na-eji DNA sperm salmon arụ ọrụ dị ka template / primer, 74 Celsius C, 30 nkeji.

Ọnọdụ mmeghachi omume

Okpomọkụ Oge mmeghachi omume Oge okirikiri
37°C 5 min 1
94°C 5 min 1
94°C Nkeji 10  40
60°C Nkeji 10

Mara:Maka sistemụ 10 µL na 20 µL, gbakwunye mmanụ ịnweta mmanụ nha nhata ma ọ bụrụ na igwe ọkụ ọkụ enweghị mkpuchi ọkụ.

Ọnọdụ mmeghachi omume PCR dịgasị iche dabere na ọnọdụ nhazi nke ndebiri, primers, na ihe ndị yiri ya.N'ime ọrụ a kapịrị ọnụ, ọ dị mkpa ịmepụta ọnọdụ mmeghachi omume kachasị mma, gụnyere okpomọkụ na-ekpo ọkụ, oge mgbatị, wdg, dị ka ọnọdụ dị iche iche dị ka ụdị template ahụ, nha nke mpempe akwụkwọ a na-atụ anya ya, usoro ntọala nke mpekere a na-agbakwụnye, na ọdịnaya GC na ogologo nke primer.

Nchekwa

-20 ± 5 Celsius C maka afọ 2 ma ọ bụ na -80 Celsius maka nchekwa ogologo oge.

  • Nke gara aga:
  • Osote:

    • Enweghị mgbama nkwalite

    1.Taq DNA Polymerase na ngwa ahụ na-efunahụ ọrụ ya n'ihi nchekwa na-ezighị ezi ma ọ bụ njedebe nke ngwa ahụ.
    Nkwanye: Kwado ọnọdụ nchekwa nke ngwa ahụ;tinyeghachi Taq DNA Polymerase kwesịrị ekwesị na sistemu PCR ma ọ bụ zụta ngwa PCR Real Time ọhụrụ maka nnwale ndị metụtara ya.

    2.E nwere ọtụtụ ihe mgbochi nke Taq DNA Polymerase na DNA template.
    Aro: Megharịa ndebiri ma ọ bụ belata ọnụọgụ ndebiri ejiri.

    3.The Mg2 + ịta adịghị adabara.
    Nkwanye: Mg2 + ntinye nke the2 × Real PCR Mix anyị na-enye bụ 3.5mM.Agbanyeghị, maka ụfọdụ primers na ndebiri pụrụ iche, ntinye Mg2+ nwere ike ịdị elu.Ya mere, ị nwere ike tinye MgCl2 ozugbo iji bulie mkpokọta Mg2+.A na-atụ aro ka ịbawanye Mg2+ 0.5mM oge ọ bụla maka njikarịcha.

    4.The PCR amplification ọnọdụ adịghị adabara, na primer usoro ma ọ bụ itinye uche na-ekwesịghị ekwesị.
    Aro: gosi izi ezi nke usoro nke primer ma emebiela primer;Ọ bụrụ na mgbama nkwuwapụta adịghị mma, gbalịa iwetulata okpomọkụ na-ekpo ọkụ ma mezie ntinye nke primer nke ọma.

    5. Ọnụ ọgụgụ nke template dị ntakịrị ma ọ bụ nke ukwuu.
    Nkwanye: Mee template linearization gradient dilution, wee họrọ mkpokọta template nwere mmetụta PCR kacha mma maka nnwale PCR oge.

    NTC nwere oke fluorescence uru

    1.Reagent mmetọ mere n'oge ọrụ.
    Nkwanye: Dochie na ọhụrụ reagents maka ezigbo oge PCR nnwale.

    2.Contamination mere n'oge nkwadebe nke usoro mmeghachi omume PCR.
    Nkwanye: Were usoro nchebe dị mkpa mgbe ị na-arụ ọrụ, dị ka: iyi uwe latex, iji ntu pipette nwere nzacha, wdg.

    3.The primers na-eweda n'ala, na mmebi nke primers ga-eme ka ndị na-abụghị kpọmkwem amplification.
    Aro: Jiri SDS-PAGE electrophoresis chọpụta ma ọ̀tụ̀tụ̀tụ̀ ihe ndị e ji emepụta ihe na-emebi emebi, ma jiri primers ọhụrụ dochie ha maka nnwale PCR Real Time.

    Primer dimer ma ọ bụ nkwalite na-abụghị nke akọwapụtara

    1.The Mg2 + ịta adịghị adabara.
    Nkwanye: Mg2 + ntinye uche nke 2 × Real PCR EasyTM Mix anyị na-enye bụ 3.5 mM.Agbanyeghị, maka ụfọdụ primers na ndebiri pụrụ iche, ntinye Mg2+ nwere ike ịdị elu.Ya mere, ị nwere ike tinye MgCl2 ozugbo iji bulie mkpokọta Mg2+.A na-atụ aro ka ịbawanye Mg2+ 0.5mM oge ọ bụla maka njikarịcha.

    2.The PCR annealing okpomọkụ dị oke ala.
    Aro: Mee ka PCR annealing okpomọkụ site 1℃ ma ọ bụ 2℃ oge ọ bụla.

    3.The PCR ngwaahịa dị ogologo.
    Nkwanye: Ogologo ngwaahịa PCR Real Time kwesịrị ịdị n'etiti 100-150bp, ọ bụghị karịa 500bp.

    4.The primers na-eweda n'ala, na nbibi nke primers ga-eduga na ọdịdị nke kpọmkwem mmụba.
    Aro: Jiri SDS-PAGE electrophoresis chọpụta ma ọ̀tụ̀tụ̀tụ̀ ihe ndị e ji emepụta ihe na-emebi emebi, ma jiri primers ọhụrụ dochie ha maka nnwale PCR Real Time.

    5.The PCR usoro na-ekwesịghị ekwesị, ma ọ bụ usoro dị oke obere.
    Aro: Sistemụ mmeghachi omume PCR pere mpe ga-eme ka nchọta nke ọma belata.Ọ kacha mma iji usoro mmeghachi omume nke akụrụngwa PCR ọnụọgụ tụrụ aro iji megharịa nnwale PCR Real Time.

    Nkwughachi nke ụkpụrụ ọnụọgụgụ adịghị mma

    1. The ngwá bụ malfunctioning.
    Aro: Enwere ike inwe mperi n'etiti oghere PCR ọ bụla nke ngwaọrụ ahụ, na-ebute mmeghari na-adịghị mma n'oge njikwa okpomọkụ ma ọ bụ nchọpụta.Biko lelee dị ka ntuziaka nke ngwa kwekọrọ.

    2.The sample ịdị ọcha adịghị mma.
    Nkwanye: Ihe nlele na-adịghị ọcha ga-eduga na mmeghari nke nnwale ahụ na-adịghị mma, nke gụnyere ịdị ọcha nke template na primers.Ọ kacha mma imegharị ndebiri ahụ, yana SDS-PAGE na-asachapụ ihe ndị ahụ.

    3.The PCR usoro nkwadebe na oge nchekwa dị ogologo.
    Aro: Jiri ezigbo oge PCR usoro maka PCR nnwale ozugbo nkwadebe, na ahapụla ya n'akụkụ ruo ogologo oge.

    4.The PCR amplification ọnọdụ adịghị adabara, na primer usoro ma ọ bụ itinye uche na-ekwesịghị ekwesị.
    Aro: gosi izi ezi nke usoro nke primer ma emebiela primer;Ọ bụrụ na mgbama nkwuwapụta adịghị mma, gbalịa iwetulata okpomọkụ na-ekpo ọkụ ma mezie ntinye nke primer nke ọma.

    5.The PCR usoro na-ekwesịghị ekwesị, ma ọ bụ usoro dị oke obere.
    Aro: Sistemụ mmeghachi omume PCR pere mpe ga-eme ka nchọta nke ọma belata.Ọ kacha mma iji usoro mmeghachi omume nke akụrụngwa PCR ọnụọgụ tụrụ aro iji megharịa nnwale PCR Real Time.

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