I-Mutagenesis Kit eqondiswe ngokushesha esizeni

Ukuguquka kwesiza esisodwa esisheshayo noma ukuguqulwa kwamasayithi amaningi kuhlobo lwenhloso ku-vector ekhonjiwe.

I-mutagenesis eqondiswe kusayithi ku-vitro iyindlela ebalulekile yokuhlola emikhakheni ehlukahlukene ye-biology nemithi, esetshenziswa kakhulu ukuguqula nokwandisa izinhlobo zofuzo ezihlosiwe, ukuhlola izindawo zokulawula zabagqugquzeli, kanye nokufunda ubudlelwano obuyinkimbinkimbi phakathi kwesakhiwo samaprotheni nomsebenzi. Ikhithi isebenzisa ubuchwepheshe bamanje obuholayo ukwenza ngqo ukuguqulwa kwesiza okukodwa, ukuguqulwa kwamasayithi amaningi kanye nokufakwa noma ukususwa kokushintsha kwesakhi sofuzo. Izinga lokuguqulwa kokushintshwa kwesayithi elilodwa lingafinyelela ngaphezu kwe-90%. Ngaphezu kwalokho, ngokungafani namakhithi wendabuko wokuguqula izinto adinga imijikelezo eminingi ye-PCR, i-sub-cloning nezinye izinyathelo ezidla isikhathi nezisebenza kanzima, ukusebenza kwekhithi kulula, futhi kudingeka izinyathelo ezine kuphela ukwakha uhlobo lwe-mutant.

Ikati. Cha Ukupakisha Usayizi
44992901 I-20 rxn

 

 


Imininingwane yomkhiqizo

Imibuzo evame ukubuzwa

Amathegi womkhiqizo

Izici

■ Ilula futhi iyashesha: Ikhithi isebenzisa ubuchwepheshe bokukhulisa i-plasmid non-strand. Kudinga kuphela izinyathelo ezi-4 zokubona inguquko isuka ohlotsheni lwasendle iye ekuxakekeni okuguqukayo, ngaphandle kwezinyathelo ezidla isikhathi nezisebenza kanzima ezinjengemijikelezo eminingi ye-PCR kanye ne-sub-cloning.
■ I-primer esebenza kahle kakhulu: Ikhithi isebenzisa umthetho wokuqamba okumbalwa okugqagqene, ukuze ama-plasmid amaningi aguqukile atholakale ngokukhulisa.
■ Kusebenza kabanzi: Ikhithi ayikwazi ukwenza kuphela ukuguqulwa kwesayithi elilodwa, kepha futhi nokuguqulwa kwamasayithi amaningi. Ingaguqula amasayithi angafika kwangu-5.
■ Ukuzivumelanisa nezimo okuqinile: Ikhithi ingenza ukuguqulwa okuqondiswe kusayithi kuma-plasmid ngosayizi omkhulu ka-10 kb, ngokuyisisekelo ehlanganisa wonke ama-plasmids asetshenziswa kakhulu.
■ Izinga lokuguqulwa okuphezulu: ikhithi inomsebenzi wokugaywa kabili kwamathempulethi e-methylated plasmid in vitro and in vivo, aqinisekisa izinga lokuguquka kwezinga eliphakeme.

Isethaphu-Reaction Reaction Setup ne-PCR Program

■ Ekushintsheni okukodwa kokuqala kwamasayithi amaningi, izinga lokuguqula izinguquko lizoba lincane kunalelo lokuguqulwa kwesayithi elilodwa ngenxa yenani elikhulile lezindawo eziguqula isimo. Ngokuya ngemininingwane yethu yokuhlola, lapho inani lezindawo eziguqula izakhi zofuzo lifinyelela ku-5, isilinganiso esihle sokuguqula izokwehliselwa ku-50%. Ngakho-ke, kulokhu, kunconywa ukwandisa inani lama-clones aqinisekisiwe.
■ Ikhithi isekela ukuguqulwa kwamasayithi amaningi, ukuze ukuhlolwa koguquko kwenziwe ngasikhathi sinye ebangeni elibanzi lezakhi zofuzo. Umkhawulo ophezulu wenani lezindawo zokuguqula isimo usengu-5.
■ Kuphakanyiswa ukuthi ama-plasmids wokulawula kanye nama-primer anikezwe ku-kit kufanele asetshenziswe lapho kwenziwa izivivinyo ezintsha zokuguqula izakhi ukuze kube lula ukuhlaziywa kwezinkinga zokuhlola.

Fast Site-Directed Mutagenesis Kit Fast Site-Directed Mutagenesis Kit

Yonke imikhiqizo ingenziwa ngezifiso i-ODM / OEM. Ngemininingwane,sicela uchofoze i-Customized Service (ODM / OEM)


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    Q: Awekho amabhendi wokukhulisa

    Isifanekiso se-A-1

    ■ Ithempulethi iqukethe ukungcola kwamaprotheni noma ama-Taq inhibitors, njll. - —Purify DNA template, susa ukungcola kwamaprotheni noma ukhiphe i-DNA template ngamakhithi okuzihlanza.

    ■ Ukwehlukaniswa kwethempulethi akuphelele ——Kwandisa ngokufanele ukushisa kwama-denaturation futhi kwandise isikhathi se-denaturation.

    ■ Ukuwohloka kwesifanekiso ——Lungisa kabusha ithempulethi.

    I-A-2 Primer

    ■ Izinga eliphansi lama-primers ——Re-synthesize the primer.

    ■ Ukuwohloka kwe-Primer ——Faka ama-primer primer aphezulu abe yivolumu encane yokulondolozwa. Gwema ukubanda okuningi nokuncibilikisa noma ukugcina isikhathi eside u-4 ° C.

    ■ Idizayini engalungile yama-primers (isb. Ubude be-primer abwenele, i-dimer eyakhiwe phakathi kwama-primers, njll.) -Redesign primers (gwema ukwakheka kwe-primer dimer nesakhiwo sesibili)

    I-A-3 Mg2+ukuhlushwa

    ■ Mg2+ ukuminyana kuphansi kakhulu —— Khulisa ngokufanele uMg2+ ukuhlushwa: Lungiselela iMg2+ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile2+ ukugxila kuthempulethi ngayinye nakuqala.

    Ukushisa kwe-A-4 Annealing

    The Ukushisa okuphezulu kokunciphiswa komthelela kuthinta ukubopha kwe-primer ne-template. - - Nciphisa ukushisa okunciphisayo futhi wenze ngcono isimo nge-gradient ka-2 ° C.

    Isikhathi se-A-5 Sesandiso

    ■ Isikhathi esifushane sokunweba — - Khulisa isikhathi sokunweba.

    Umbuzo: Ukuthi kunamanga

    I-Phenomena: Amasampula amabi nawo akhombisa amabhendi wokulandelana okuqondiwe.

    Ukungcola kwe-A-1 kwe-PCR

    ■ Ukungcola kwesiphambeko sokulandelana okuqondiwe noma imikhiqizo yokukhulisa amandla ——Nakekela ukuthi ungafaki isampuli ngesampula equkethe ukulandelana kwethagethi kusampula engeyinhle noma uchithe iphume kushubhu le-centrifuge. Ama-reagents noma okokusebenza kufanele kwenziwe ngokuzenzakalela ukuqeda ama-nucleic acid akhona, futhi ubukhona bokungcola kufanele kunqunywe ngokuhlolwa kokulawulwa okungalungile.

    ■ Ukungcola okuyisenzo ——Faka ama-reagents bese uwagcina lapho kushisa okuncane.

    I-A-2 Primer

    ■ Mg2+ ukuminyana kuphansi kakhulu —— Khulisa ngokufanele uMg2+ ukuhlushwa: Lungiselela iMg2+ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile2+ ukugxila kuthempulethi ngayinye nakuqala.

    ■ Idizayini yokuqala engafanele, nokulandelana kwempokophelo kune-homology ngokulandelana okungeyona eyenhloso. ——Kwakha kabusha ama-primers.

    Q: Ukukhulisa okungacacisiwe

    I-Phenomena: Amabhendi wokukhulisa we-PCR awahambelani nosayizi olindelekile, kungaba mikhulu noma mincane, noma kwesinye isikhathi womabili amabhendi okukhulisa kanye namaqembu wokukhulisa angaqondile.

    I-A-1 Primer

    ■ Ukucaciswa okungafanelekile kokuqala

    ——Kwakha kabusha isiqalo.

    ■ Ukuhlungwa kwe-primer kuphakeme kakhulu — -Kwandisa ngokufanele ukushisa kwe-denaturation futhi kwandise isikhathi se-denaturation.

    I-A-2 Mg2+ ukuhlushwa

    ■ UMg2+ ukuminyana kuphakeme kakhulu —— Nciphisa kahle ukuhlushwa kwe-Mg2 +: Lungiselela iMg2+ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile2+ ukugxila kuthempulethi ngayinye nakuqala.

    I-A-3 Thermostable polymerase

    ■ Inani le-enzyme eyeqile - - Nciphisa inani le-enzyme ngokufanele ngezikhathi ezithile zika-0.5 U.

    Ukushisa kwe-A-4 Annealing

    ■ Izinga lokushisa elinciphisayo liphansi kakhulu ——Kwandisa ngokufanele ithempelesha yokuncisha noma ukusebenzisa indlela yokuncisha izigaba ezimbili

    Imijikelezo ye-A-5 PCR

    ■ Imijikelezo eminingi kakhulu ye-PCR —— Nciphisa inani lemijikelezo ye-PCR.

    Q: Ama-Patchy noma ama-smear bands

    I-A-1 Primer—— Okucacile okungekuhle—— Yakha kabusha i-primer, shintsha ukuma nobude be-primer ukuthuthukisa ukucaciswa kwayo; noma wenze i-PCR ehlanganisiwe.

    I-A-2 Template DNA

    ——Isifanekiso asihlanzekile —Hlanza ithempulethi noma ukhiphe i-DNA enezikhwama zokuhlanzwa.

    I-A-3 Mg2+ ukuhlushwa

    - —Mg2+ ukugxilisa ingqondo kuphakeme kakhulu ——Ukunciphisa kahle uMg2+ ukuhlushwa: Lungiselela iMg2+ ukugxila ngochungechunge lokuphendula kusuka ku-1 mM kuye ku-3 mM ngesikhawu esingu-0.5 mM ukuthola iMg efanelekile2+ ukugxila kuthempulethi ngayinye nakuqala.

    I-A-4 dNTP

    —— Ukuhlungwa kwama-dNTP kuphakeme kakhulu —— Nciphisa ukuminyana kwe-dNTP ngokufanele

    Ukushisa kwe-A-5 Annealing

    ——Ukushisa okuncishisayo okuphansi impela —— Kukhuphula kahle ukushisa okuncishisayo

    Imijikelezo engu-A-6

    —Imijikelezo eminingi kakhulu —— Yandisa inani lomjikelezo

    Q: Mangaki ithempulethi ye-DNA okufanele ingezwe ku-50 μl system reaction reaction?
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    Q: Ungazikhulisa kanjani izingcezu ezinde?

    Isinyathelo sokuqala ukukhetha i-polymerase efanelekile. I-Taq polymerase ejwayelekile ayikwazi ukufundwa ngenxa yokuntuleka komsebenzi we-3'-5 'wokuxolelwa, futhi ukungafani kahle kuzonciphisa kakhulu ukusebenza kwezingcezu. Ngakho-ke, i-Taq polymerase ejwayelekile ayikwazi ukukhulisa ngempumelelo izingcezu ezihlosiwe ezinkulu kune-5 kb. I-Taq polymerase enokuguqulwa okukhethekile noma okunye ukuthembeka okuphezulu kwe-polymerase kufanele kukhethwe ukuthuthukisa ukusebenza kahle kokunwetshwa nokuhlangabezana nezidingo zokukhulisa isiqeshana eside. Ngaphezu kwalokho, ukukhuliswa kwezingcezu ezinde kudinga nokulungiswa okuhambisanayo komklamo wokuqala, isikhathi sokudlulisa isikhathi, isikhathi eseluliwe, i-pH yesikhondlakhondla, njll. Ngokuvamile, ama-primers ane-18-24 bp angaholela esivunweni esingcono. Ukuvikela ukulimala kwethempulethi, isikhathi sokudonswa kwenani elingu-94 ° C kufanele sehliswe lifike kumasekhondi angama-30 noma ngaphansi ngomjikelezo ngamunye, nesikhathi sokukhuphuka kwamazinga okushisa siye ku-94 ° C ngaphambi kokukhulisa amandla kufanele kube ngaphansi kweminithi elilodwa. Ngaphezu kwalokho, ukusetha izinga lokushisa lokunwebeka cishe ku-68 ° C nokuklama isikhathi sesandiso ngokuya ngesilinganiso se-1 kb / min kungaqinisekisa ukukhuliswa okusebenzayo kwezingcezu ezinde.

    Q: Ungakuthuthukisa kanjani ukwethembeka kokukhulisa kwe-PCR?

    Izinga lephutha lokukhulisa i-PCR lingehliswa ngokusebenzisa ama-polymerase e-DNA ahlukahlukene ngokuthembeka okuphezulu. Kuwo wonke ama-polymerase eTaq DNA atholakele kuze kube manje, i-Pfu enzyme inezinga lephutha eliphansi kakhulu nokuthembeka okuphezulu (bheka ithebula elihlanganisiwe). Ngaphezu kokukhethwa kwe-enzyme, abacwaningi bangaqhubeka banciphise izinga lokuguqulwa kwe-PCR ngokwenza ngcono izimo zokuphendula, kufaka phakathi ukwakheka kwe-buffer, ukuminyana kwe-polymerase esetshenziswayo nokwandisa inombolo yomjikelezo we-PCR.

    Bhala umyalezo wakho lapha bese uwuthumela kithi