I-FastKing RT Kit (Nge-gDNase)

Funda kahle zonke izinhlobo zokulandelana futhi ukhombe ngokunembile amathempulethi enqwaba ephansi.

I-FastKing RT Kit (ene-gDNase) uhlelo olusebenzayo, oluzinzile nolusheshayo lokubuyisela emuva olukwazi ukususa ukungcoliswa kwe-genomic DNA. Ikhithi iqukethe i-gDNase yokususa kahle i-genomic DNA, kepha ingathinti ikhwalithi ye-cDNA. I-Enzyme esebenza kahle kakhulu ebuyisela emuva i-FastKing RT ilungele izifanekiso ze-RNA ezinokuqukethwe okujwayelekile noma okuphezulu kwe-GC kanye nesakhiwo esiyinkimbinkimbi sesibili kanye nokumelana nengcindezi.

Ikati. Cha Ukupakisha Usayizi
4992223 I-25 rxn
4992224 I-100 rxn
4992250 I-1000 rxn

Imininingwane yomkhiqizo

Isibonelo sokuhlola

Imibuzo evame ukubuzwa

Amathegi womkhiqizo

Izici

■ Ukusebenza kahle okuphezulu: I-FastKing RT Enzyme iguqulwa nge-hydrophobic motif, ngokusebenza kahle kwe-RT ngaphezu kwama-95%.
■ Ukuzwela: Uma izifanekiso ezingaphansi kwezingu-1 ng zingakhonjwa ngokunembile.
■ Ukumelana: Iyakwazi ukuloba okubuyela emuva kwezifanekiso eziyinkimbinkimbi, nokumelana ngokuphelele nokungcola.
■ Flexible: Ukususwa kwe-Genomic DNA nokubhalwa phansi okuphindwe kabili kwaqedwa ngokwehlukana. Ama-Primers ayexubaniswe ngokwahlukana ethubhu, eguquguqukayo ukushintsha amanye ama-primers.

Ukucaciswa

Uhlobo: I-Gene modified reverse transcriptase, gDNase
Izinqubo: Izinyathelo ezimbili (ukususwa kwe-genomic DNA ne-RT)
Ukusebenza kahle kwe-RT:> 95%
Isifanekiso: 1 ng- 2 μg
Isikhathi sokusebenza: ~ 21 min
Izicelo: I-cDNA ebhaliwe ebhaliwe ingasetshenziswa ku-PCR ejwayelekile, i-Real time PCR, ukwakhiwa kwelabhulali ye-cDNA.

Ukusabela okungu-21 min kwithumbu elilodwa

Kuthatha kuphela ama-21 min ukuqedela ukususwa kwe-gDNA nenqubo yokubhala ngokuhlehlisa esebenza kahle kushubhu efanayo ngaphandle kokufaka esikhundleni se-reaction reaction kanye nenqubo yokwelashwa kwe-DNase I ezimele. Uma kuqhathaniswa nendlela yendabuko edinga ukusebenza kwezinyathelo eziyi-12 nokuphendula okungu-140 min, yenza lula kakhulu izinyathelo zokusebenza futhi isindise isikhathi esiningi sokusebenza.

21 min reaction in one-tube

Ikhwalithi evelele yeKing RTase

—I-Ultra-high reverse reverse transcription
——Ukusebenza ngokucophelela kokubhaliwe kungaphezu kwama-95%
I-reverse transcriptase ejwayelekile inekhono lokubhala eliphindayo elingu-40-60%, futhi isivuno se-cDNA singakhuphuka ngenani eliphakeme lokulayisha le-RNA. I-King reverse transcriptase ingafinyelela ukuhleleka kokubhalwa phansi okungaphezulu kuka-95% ngenxa yokuhlangana kwayo okuhlukile okuphezulu kwezifanekiso ze-RNA. Ngakho-ke, ukuhlolwa okulandelayo kunganeliswa ngaphandle kwesidingo semali enkulu yokufakwa kwe-RNA, okusindisa i-RNA futhi kunike amandla ukuhlanzeka okuphezulu nokuvunwa okuphezulu kwe-cDNA.
Outstanding quality of King RTase

Funda kalula ngezifanekiso eziyinkimbinkimbi

——Funda kalula nge-GC ephezulu nezifanekiso eziyinkimbinkimbi
I-RNA eyodwa enezintambo inezinhlobonhlobo zezifunda eziyinkimbinkimbi zesakhiwo ngenxa yokuhlangana kwe-hydrogen phakathi kwemicu. I-reverse transcriptase ejwayelekile ingaholela ekunqanyulweni kokubhalwa phansi okuphambene nomthetho lapho ihlangabezana nesakhiwo esiyinkimbinkimbi, ngakho-ke ayikwazi ukuqedela ngempumelelo ukuhlanganiswa kwe-cDNA. Kodwa-ke, isizukulwane esisha seKing reverse transcriptase sinesizinda esihlukile, esingaqeda isibopho se-hydrogen phakathi kwezintambo ze-RNA, ngaleyo ndlela kuvuleke isakhiwo sesibili esiyinkimbinkimbi se-RNA nokuqinisekisa ukubhalwa phansi okubushelelezi.

Easily read through complex templates

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


  • Langaphambilini
  • Olandelayo:

  • product_certificate04 product_certificate01 product_certificate03 product_certificate02
    ×
    Experimental Example Iqembu 1: Ukuguqula umbhalo ngaphandle kokwelashwa kwe-gDNase; Iqembu 2: Akukho ukwelashwa kwe-gDNase futhi akukho okubhaliwe okuphambene nalokho; Iqembu 3: Ukubuyisela emuva umbhalo ngemuva kokwelashwa kwe-gDNase; Iqembu 4: ukwelashwa kwe-gDNase ngaphandle kokuloba okuphindayo. Izindlela: Ukutholwa kwe-Fluorescence quantitative PCR ye-TNF-alpha gene (i-primer eyenzelwe ku-exon ne-cDNA noma i-genome njengethempulethi) kusetshenziswa i-1 μg Hela cell RNA (enezinsalela ze-genome) njengethempulethi. izinsalela ze-genome ku-RNA, iqembu 3 lingabonisa ngokunembile izinga leqiniso le-TNF-alpha, iqembu 1 linamaphutha emiphumeleni yokugcina yobuningi ngenxa yezinsalela ze-genome, futhi iqembu le-4 likhombisa ukuthi i-FastKing RT Kit ingasusa ngokuphelele i-DNA ye-genomic esele I-RNA.
    Experimental Example Umdwebo 1. Ukubhalwa okuguqukayo kwegundane i-RNA kwenziwa kusetshenziswa i-TIANGEN FastKing RT Kit (kwesobunxele) kanye nomkhiqizo ofanele we-Supplier A (kwesokudla), lapho-ke isakhi sofuzo seMM5 sandiswa kakhulu kusetshenziswa i-TIANGEN SuperReal PreMix Plus (SYBR Green). Ijika lokukhulisa kanye nejika lokuncibilika lahlaziywa. Okokufaka kwe-RNA kwakungu-1000 ng, 100 ng, 10 ng no-1 ng ngokulandelana. Imiphumela ikhombisa ukuthi i-TIANGEN FastKing RT Kit inenani elicacile le-transcript gradient ne-low Ct, futhi inezinzuzo ezisobala zokubhalwa phansi kwe-template ubuningi obuphansi (1 ng, umcibisholo oluhlaza okwesibhakabhaka).
    Experimental Example Umdwebo 2. Ukuguqulwa okubhaliwe kwethempulethi ejwayelekile ye-RNA (ebomvu), ithempulethi enezinsalela ezinkulu ze-phenol (oluhlaza) nethempulethi enezinsalela zotshwala (okuluhlaza okwesibhakabhaka) kwamagundane kusetshenziswa i-TIANGEN FastKing RT Kit kanye nomkhiqizo ofanele we-Supplier A ngokulandelana, zilinganise izinhlobo zofuzo ze-RNC zisebenzisa i-TIANGEN SuperReal I-PreMix Plus (i-SYBR Green), namajika okukhulisa kanye namanani we-Ct ahlaziywa. Imiphumela ikhombisa ukuthi i-TIANGEN FastKing RT Kit inenani eliphansi kunawo wonke le-Ct ngemuva kokubhalwa okuningiliziwe nokuphikiswa okuhle kakhulu kwengcindezi, futhi kunezinzuzo ezisobala zamathempulethi anensalela ephezulu yokungcola
    Q: Umkhiqizo omncane noma ongenawo we-RT-PCR

    I-A-1 RNA yehlisiwe

    ——Qondisa izinga eliphezulu le-RNA ngaphandle kokungcola. Izinto okukhishwa kuzo i-RNA kufanele zibe zintsha ngangokunokwenzeka ukuvimbela ukonakala kwe-RNA. Hlaziya ubuqotho be-RNA ku-gel esetshenzisiwe ngaphambi kokuphendula kwe-RT. Ngemuva kokukhishwa kwe-RNA, kufanele igcinwe ku-100% formamide. Uma kusetshenziswa i-RNase inhibitor, ithempelesha yokushisa kufanele ibe ngu- <45 ° C, kanti i-pH kufanele ibe ngaphansi kuka-8.0, uma kungenjalo i-inhibitor izokhipha yonke i-RNase eboshiwe. Ngaphezu kwalokho, i-RNase inhibitor kufanele ingezwe kuzixazululo eziqukethe ≥ 0.8 mM DTT.

    I-A-2 RNA iqukethe ama-inhibitors we-reverse transcript reaction

    ——Reverse transcription inhibitors ifaka i-SDS, i-EDTA, i-glycerol, i-sodium pyrophosphate, i-spermidine, i-formamide, i-guanidine usawoti, njll. Hlanganisa i-RNA yokulawula nesampuli, bese uqhathanisa isivuno nempendulo ye-RNA yokulawula ukuze uhlole ukuthi ingabe ikhona yini i-inhibitor. Geza imvula ye-RNA nge-70% (v / v) ethanol ukususa ama-inhibitors.

    I-A-3 annealing eyanele yama-primers asetshenziselwa ukuhlanganisa umucu wokuqala we-cDNA

    - Nquma ukuthi i-annealing lokushisa kufanelekile kuma-primers asetshenziswe ekuhlolweni. Ngama-hexamers angahleliwe, kunconywa ukuthi ugcine izinga lokushisa liku-25 ° C ngemizuzu eyi-10 ngaphambi kokufinyelela izinga lokushisa lokuphendula. Kuma-primers aqondene nezakhi zofuzo (GSP), zama enye i-GSP, noma ushintshele ku-oligo (dT) noma i-hexamer engahleliwe.

    Inani elincane le-A-4 lokuqala i-RNA

    - Khulisa inani le-RNA. Ngamasampula e-RNA angaphansi kuka-50 ng, i-0.1 μg kuya ku-0.5 μg i-acetyl BSA ingasetshenziswa ekuhlanganisweni kokuqala kwe-strand cDNA

    A-5 Ukulandelana okuqondiwe akuboniswa kuzicubu ezihlaziyiwe.

    ——Zama ezinye izicubu.

    Ukusabela kwe-A-6 PCR kwehluleka

    ——Kwezinyathelo ezimbili i-RT-PCR, ithempulethi ye-cDNA esinyathelweni se-PCR ayikwazi ukudlula i-1/5 yevolumu yokuphendula.

    Q: Kuvela amabhendi angaqondile

    Ukuncishiswa okungacacisiwe kwama-primers nama-templates

    —— Ukuphela kuka-3'kokuqala kwama-primers akufanele kube ne-2-3 dG noma i-dC. Sebenzisa ama-primers akhethekile we-Gene ku-strand synthesis yokuqala esikhundleni sama-primers angahleliwe noma i-oligo (dT). Sebenzisa ukushisa okuphezulu kokuncisha emijikelezweni embalwa yokuqala, bese izinga lokushisa elingaphansi elincishisiwe. Sebenzisa i-hot-start Taq DNA polymerase ye-PCR ukuthuthukisa ukucaciswa kokuphendula.

    Idizayini engalungile ye-A-2 yama-primers aqondene nezakhi zofuzo

    - Landela imigomo efanayo yokuklama i-amplification primer design.

    I-A-3 RNA ingcoliswe yi-genomic DNA

    —Thola i-RNA nge-PCR-grade DNase I. Setha ukusabela kokulawula ngaphandle kokuloba okubuyela emuva ukuthola ukungcola kwe-DNA.

    Ukwakhiwa kwe-primer dimer

    Ama-primers okuklama ngaphandle kokulandelana okuhambisanayo ekugcineni kuka-3.

    A-5 Mg ephakeme kakhulu2+ ukuhlushwa

    —— Lungiselela uMg2+ ukugxila kuthempulethi ngayinye nokuhlanganiswa kokuqala

    I-A-6 Ingcoliswe nge-DNA yangaphandle

    —— Sebenzisa amathiphu amelana ne-aerosol nama-enzyme e-UDG.

    Q: Ama-Smear bands

    A-1 Okuqukethwe komkhiqizo we-strand wokuqala kuphezulu kakhulu

    - - Nciphisa inani lomkhiqizo wokuqala we-strand kusinyathelo esivamile se-PCR reaction.

    Inani elingu-A-2 eliphakeme kakhulu ekuphenduleni kwe-PCR

    - - Nciphisa okokufaka kokuqala.

    A-3 Imijikelezo eminingi kakhulu

    Lungiselela izimo zokuphendula ze-PCR futhi unciphise inombolo yomjikelezo we-PCR.

    A-4 Ukushisa okuphansi kakhulu

    —Ukwandisa izinga lokushisa lokunciphisela ukuvimbela ukuqalisa nokunweba okungacacisiwe.

    I-A-5 Ukukhulisa okungacaciswanga kwezingcezu ze-oligonucleotide ezikhiqizwe ukonakala kwe-DNase kwe-DNA —— Khipha i-RNA esezingeni eliphezulu ukuvimbela ukungcoliswa kwe-DNA.

    Q: Ungawakhetha kanjani ama-primers we-RT-PCR?

    I-RT-PCR ukubuyisela emuva ukubhala phansi i-RNA ibe yi-cDNA, bese usebenzisa i-cDNA ebhaliwe ebuyiselwe njengesifanekiso sokuphendula kwe-PCR ukukhulisa isiqeshana esiqondisiwe. Khetha ama-primers angahleliwe, i-Oligo dT kanye nama-primers aqondene nezakhi zofuzo ngokuya ngezimo ezithile zesilingo. Onke ama-primers angenhla angasetshenziselwa i-eukaryotic cell mRNA ngaphandle kwesakhiwo se-hairpin.

    I-Random primer: Ifanele i-RNA ende enesakhiwo se-hairpin, kanye nazo zonke izinhlobo ze-RNA ezinjenge-rRNA, mRNA, tRNA, njll. Zisetshenziselwa ukuphendula kwe-RT-PCR kwesifanekiso esisodwa.

    I-Oligo dT: Ifanele i-RNA ene-PolyA tailing (i-prokaryotic RNA, i-eukaryotic i-Oligo dT rRNA ne-tRNA ayinayo imisila ye-PolyA). Ngoba i-Oligo dT iboshelwe kumsila wePolyA, ikhwalithi yamasampuli e-RNA iyadingeka ukuthi ibe phezulu, futhi noma inani elincanyana lokwehlisa izinga lizokwehlisa kakhulu inani lokuhlanganiswa okugcwele kwe-cDNA.

    I-primer ekhethekile ye-Gene: Ihambisana nokulandelana kwethempulethi, efaneleke ezimeni lapho ukulandelana kwempokophelo kwaziwa.

    Q: Ungaqinisekisa kanjani ukuphumelela kwe-RNA reverse transcription ku-strand cDNA yokuqala?

    Kunezindlela ezimbili:

    1. Indlela yereferensi yangaphakathi: Ngokombono, i-cDNA izingcezu ze-DNA zobude obuhlukile, ngakho-ke umphumela we-electrophoresis yi-smear. Uma ubuningi be-RNA buphansi, awukho umkhiqizo ozobonakala ku-electrophoresis, kepha lokhu akusho ukuthi awukho umkhiqizo ozokwandiswa yi-PCR. Ngokuvamile, ireferensi yangaphakathi ingasetshenziselwa ukuthola i-cDNA. Uma ireferensi yangaphakathi inemiphumela, ikhwalithi ye-cDNA ingaqinisekiswa ngokuyisisekelo (ezimweni ezimbalwa, uma isiqeshana sofuzo esihlosiwe side kakhulu, kungahle kube nokuhlukile).

    2. Uma kukhona ufuzo olwaziwe olwandiswa yilesi sifanekiso, lungaqinisekiswa ngabokuqala balesi sakhi. Ukukhuliswa kwesethenjwa sangaphakathi akusho ukuthi ayikho inkinga nge-cDNA. Ngoba ireferensi yangaphakathi inenqwaba ye-cDNA, kulula ukuyikhulisa. Uma i-cDNA yehliswa ngokwengxenye ngenxa yezizathu ezahlukahlukene, ngokubuka kokungenzeka, imiphumela ye-PCR yezakhi zofuzo eziqondiwe ngobuningi izothinteka kakhulu. Ngenkathi ireferensi yangaphakathi isaphezulu ngobuningi, ukukhulisa amandla kungenzeka kungathinteki.

    Q: I-RT-PCR inganweba izakhi zofuzo zangaphakathi kodwa ingabhekisi izakhi zofuzo

    Ukuwohloka kancane kwe-RNA. Thola ubuqotho bese uhlanza i-RNA

    Okuqukethwe kwe-RNA yezinhlobo ezahlukahlukene kungahluka, kepha ngokujwayelekile, inani eliphelele le-RNA kufanele libe namabhande amabili acacile we-28S kanye ne-18S ku-gel electrophoresis, futhi ukukhanya kwebhande langaphambili kufanele kuphakame ngokuphindwe kabili kunokwalokhu okugcina. Ibhendi le-5S likhombisa ukuthi i-RNA yehlisiwe, futhi ukukhanya kwayo kuyalingana nezinga lokwehla. Ukukhuliswa ngempumelelo kwesethenjwa sangaphakathi akusho ukuthi ayikho inkinga nge-RNA, ngoba ireferensi yangaphakathi inenqwaba ephezulu, i-RNA ingakhuliswa inqobo nje uma ukonakala kungabi kubi. I-OD260/ OD280isilinganiso se-RNA emsulwa esilinganiswe nge-spectrophotometer kufanele sibe phakathi kuka-1.9 no-2.1. Inani elincane lokungcola kwamaprotheni ku-RNA kuzonciphisa isilinganiso. Uma nje inani lingaphansi kakhulu, i-RT ngeke ithinteke. Okubaluleke kakhulu kwi-RT ubuqotho be-RNA.

    Q: Ungaqinisekisa kanjani impumelelo ye-RT?

    Ukunwetshwa kofuzo lwesithenjwa sangaphakathi kungakhombisa kuphela ukuthi i-RT iphumelele, kepha akuhlobene neze nekhwalithi yomucu we-cDNA. Ngoba izingcezu zezethenjwa zangaphakathi ngokuvamile zincane ngosayizi futhi ziveza okukhulu, kulula ukuphumelela ekubhaleni okuphindayo. Kodwa-ke, ubukhulu nokuvezwa kohlobo oluhlosiwe kuyahlukahluka kuye ngezakhi zofuzo. Ikhwalithi ye-cDNA ayikwazi ukwahlulelwa kuphela ngesethenjwa sangaphakathi ikakhulukazi izingcezu ezihlosiwe ezinde kune-2 kb.

    Amanye amasampula anezakhiwo eziyinkimbinkimbi zesibili, noma anokuqukethwe okunothile kwe-GC, noma ayigugu ngobuningi obuphansi. Kulezi zimo, kufanele kukhethwe i-reverse transcriptase efanele ngosayizi wocezu lwenhloso nesampula. Okwezifanekiso ze-RNA ezinokuqukethwe okuphezulu kwe-GC nokwakheka okuyinkimbinkimbi kwesekondari, kunzima ukuvula isakhiwo sesibili emazingeni aphansi okushisa, noma nge-reverse transcriptase ejwayelekile. Kula mathempulethi, i-Quant Reverse Transcriptase ingakhethwa, ngoba ukusebenza kwayo okuphambene nomqondo ngokusobala kungcono kunalokho kwe-M-MLV series reverse transcriptase, engaguqula ukubhalwa kwamathempulethi ahlukahlukene e-RNA kahle futhi ibhale i-RNA ibe yi-cDNA strand yokuqala ize ifike ezingeni eliphezulu. Lapho usebenzisa i-reverse reverse transcriptase kit, uhlelo lwama-20 μl lungaguqula ngempumelelo kuphela ukubhala okungu-1 μg we-RNA ephelele. Sicela unake umthamo omkhulu we-RT wekithi. Uma ithempulethi ingezwe ngokweqile, ukuloba okuphindayo kuzokwenzela i-RNA ngobuningi obuphezulu. Ngakho-ke, kungcono ukuthi ungadluli umthamo omkhulu wesistimu.

    Q: I-RT-PCR ayikwazi ukukhulisa uhlobo lwesithenjwa sangaphakathi

    A-1 Thola ukuthi i-RNA yehliswe isithunzi kakhulu nokuthi i-RT iphumelele yini

    Ngokuvamile, isizathu sokwehluleka kokukhuliswa kwereferensi yangaphakathi kuvame ukubangelwa ukwehla okukhulu kwe-RNA. Esinye isizathu esingaba khona ukwehluleka kokuloba okuphindayo. Isethenjwa sangaphakathi asinakusetshenziswa njengezinga lokwahlulela ikhwalithi ye-cDNA single strand, kepha ingasetshenziswa njengezinga elijwayelekile lokwahlulela ukuthi ukuloba okuphindayo kuyaphumelela uma ingekho inkinga yekhwalithi ye-RNA. Into ebaluleke kakhulu kunqubo yokubhala okuphindayo ukugcina ukushisa okungaguquguquki kanye nohlelo lokuphendula njalo ukuze kuthuthukiswe ukusebenza kahle kokuphendula.

    I-A-2 Nquma ukuthi ingabe iziqalo zokukhulisa izakhi zofuzo zereferensi yangaphakathi zinokwethenjelwa futhi uma kunezinkinga ngama-reagents asetshenziswa ku-PCR.

    Q: Lapho uthola izinga le-RNA le-quantification ehlobene, kuyadingeka yini ukuthi uguqule ukuloba kwakho kube yi-cDNA ngaphansi kwesimo sokuthi ukuhlushwa kwe-RNA kwesampula ngayinye kuyafana?

    Ukuze kwenziwe i-quantification ehlobene, i-RNA kufanele ibalwe ngaphambi kokubhalwa phansi okuphindwayo, okudingekayo nakuma-kits amaningi wokubhala okuphindayo, ngokwesibonelo, ulinganise okokufaka kwe-RNA njenge-1 μg. Njengoba i-cDNA ebhalwe phansi iyisixazululo esihlanganisiwe, kufaka phakathi i-RNA, i-oligo dT, i-enzyme, i-dNTP, kanye nensalela encane ye-DNA, ukuphambuka kuzobangelwa, ngakho-ke akunakwenzeka ukukala ngokunembile i-cDNA. Ngakho-ke, i-quantification ye-RNA iyadingeka. Uma kubhekwa ukusebenza kwe-transcript okuphindayo kuyafana phakathi kwamasampuli ahlukahlukene, inani le-cDNA elitholakele kufanele lifane, futhi ukuhlaziywa kwenani kungakhombisa ukuqhathaniswa kwamazinga okuveza izakhi zofuzo ezahlukahlukene ngenani elifanayo le-RNA ephelele. Lapho wenza i-PCR yokulinganisa i-fluorescence ehambisanayo, i-cDNA yokulinganisa kungenzeka ingadingeki ngemuva kokubhalwa okuphindayo ngoba isakhi sangaphakathi senkomba singenziwa njengesethenjwa.

    Q: Kungenzeka yini ukuhlehlisa okulotshiwe izingcezu ezinde?

    Ihlobene kakhulu nezakhi zofuzo, futhi ukubhalwa phansi kwesiqeshana eside akunakwenzeka ezinhlotsheni eziningi zofuzo. Okokuqala, ukusebenza kahle kokuloba okuphindayo kuncane kakhulu kunokwe-PCR. Okwesibili, indawo ecebile ye-GC nokwakheka kwesibili kwezakhi zofuzo eziningi kuvimbela kokubili ukubhalwa phansi kwe-reverse ne-PCR. Ekugcineni, ukuthembeka nokukhulisa ukusebenza kwe-PCR kunzima ukukuqinisekisa ngasikhathi sinye. Ngenqubo yokubhalwa phansi okuphindayo, akekho umuntu ongaqinisekisa ukuthi uthola izingcezwana ezinde zezakhi zofuzo eziphansi, ikakhulukazi usebenzisa i-oligo dT. Ngokuqondene ne-5 'UTR ene-GC eningi, kunzima kakhulu. Ngakho-ke, kuseseyindlela enengqondo yokuhlehlisa okulotshiweyo ngama-primers angahleliwe, thola amasayithi wemvelo wokuqhekeka esiqeshini esihlosiwe, ukhulise ngamasegmenti, bese wenza ukuvinjelwa kokugaywa nokuhlanganiswa. Ngokuvamile, kunzima ukukhulisa ngqo izingcezu ezinkulu kune-2 kb, kepha akunakwenzeka ngaso sonke isikhathi ukuthola: 1. Okokuqala, qinisekisa ubuqotho be-RNA / mRNA, nokukhethwa kwe-TRIZOL. I-2.M-MLV RT-PCR kit ingasetshenziswa ngqo. Nweba isikhathi sokuncipha futhi ukhulise inombolo yomjikelezo kunqubo yokukhulisa kahle. Ngenye indlela, i-PCR ehlanganisiwe ingasetshenziswa, noma yenze ukuphendula okukodwa noma okubili kuqala ngokunwetshwa ngendlela efanele nesikhathi sokunweba ngaphambi kokukhulisa okujwayelekile kwe-PCR, okungasiza ukunweba izingcezwana. Nakani ukwethembeka kwe-polymerase. I-3.Long Taq ingasetshenziswa ku-PCR ukuthola imiphumela emihle. Ukusetshenziswa kwesicelo sokuveza amaprotheni, kufanele kusetshenziswe ukuthembeka okuphezulu kwe-polymerase.

    Q: Izici zomkhiqizo we-Quant / King Reverse Transcriptase nomehluko wayo kusuka ku-TIANScript M-MLV.

    Kunezinhlobo ezimbili ze-reverse transcriptase enikezwa yi-TIANGEN: I-Quant / King RTase ne-TIANScript M-MLV. Umehluko omkhulu phakathi kwazo inani lokufaka lezifanekiso. I-Quant iyi-reverse transcriptase eyingqayizivele, eyehlukile kune-M-MLV esetshenziswa kakhulu etholakala ku-Moloney murine leukemia virus. I-Quant yi-high transactionase ephezulu esebenza kahle kakhulu evezwe ngokucophelela ngobunjiniyela i-Escherichia coli. I-Quant ilungele ukukhulisa ama-50 ng-2 μg we-RNA ngomsebenzi ophindaphindwayo wokubhala phansi kanye nesivuno esikhulu. Uma kuqhathaniswa ne-MMLV ejwayelekile noma i-AMV, isici esikhulu kakhulu se-Quant ukuthi inobuhlobo obuqinile nezifanekiso ze-RNA futhi ingaguqula amathempulethi ayinkimbinkimbi ngokubhaliwe ngaphandle kokushiswa okuphezulu kokushisa. Okwezifanekiso ezinokuqukethwe okuphezulu kwe-GC, ukusebenza ngempumelelo okuphakeme kuphezulu. Kodwa-ke, le reverse transcriptase inomsebenzi we-RNase H, ongathinta ubude bomkhiqizo we-cDNA (ofanele amathempulethi angu- <4.5 kb). Ngokuloba okujwayelekile okubuyela emuva, Kunconywa i-TIANScript MMLV reverse transcriptase. Le RTase iyi-enzyme eguquliwe enomsebenzi obuthakathaka kakhulu we-RNase H, efanelekile ukuhlanganiswa kwama-cDNA amade (> 5 kb) cDNA.

    Q: Ungakhetha kanjani phakathi kwesinyathelo esisodwa nezinyathelo ezimbili i-RT-PCR?

    Isinyathelo esisodwa sokuphindisela emuva nokukhuliswa kwe-PCR kuqedwa kushubhu efanayo ngaphandle kokuvula ikhava yeshubhu phakathi kokuhlanganiswa kwe-cDNA nokukhulisa, okusiza ukunciphisa ukungcoliswa. Njengoba wonke amasampula e-cDNA atholakalayo asetshenziselwa ukukhulisa, ukuzwela kuphakeme, ubuncane be-0.01 pg ye-RNA ephelele. Kwi-RTPCR yesinyathelo esisodwa esiphumelelayo, ama-primers aqondene nezakhi zofuzo ngokuvamile asetshenziselwa ukuqala ukuhlanganiswa kwe-cDNA. Indlela enezinyathelo ezimbili, okuyi-reverse transcript ne-PCR amplification yenziwa ngezinyathelo ezimbili. Okokuqala ukuloba okubuyela emuva kwenziwa kusuka kuthempulethi ye-RNA ukuthola i-cDNA, futhi i-cDNA etholakele ibhekene nokuphendula okukodwa noma okuningi kwe-PCR. Indlela enezinyathelo ezimbili ingasebenzisa i-oligo (dT) noma ama-primers angahleliwe ukuqondisa ukuhlanganiswa kwe-strand yokuqala ye-cDNA, futhi ingaguqula ukuloba lonke ulwazi lwe-mRNA kusuka kusampula ethile.

    Bhala umyalezo wakho lapha bese uwuthumela kithi