| dc.creator | Ramos, Andrea E. | |
| dc.creator | Muñoz, Marina | |
| dc.creator | Moreno‑Pérez, Darwin A. | |
| dc.creator | Patarroyo, Manuel A. | |
| dc.date.accessioned | 2018-12-14T13:02:55Z | |
| dc.date.available | 2018-12-14T13:02:55Z | |
| dc.date.created | 2018-12-14T13:02:55Z | |
| dc.date.issued | 2017 | |
| dc.identifier | 21910855 | |
| dc.identifier | http://repository.urosario.edu.co/handle/10336/18824 | |
| dc.description.abstract | DNA cloning is an essential tool regarding DNA recombinant technology as it allows the replication of foreign DNA fragments within a cell. pELMO was here constructed as an in-house cloning vector for rapid and low-cost PCR product propagation; it is an optimally designed vector containing the ccdB killer gene from the pDONR 221 plasmid, cloned into the pUC18 vector’s multiple cloning site (Thermo Scientific). The ccdB killer gene has a cleavage site (CCC/GGG) for the SmaI restriction enzyme which is used for vector linearisation and cloning blunt-ended products. pELMO transformation efficiency was evaluated with different sized inserts and its cloning efficiency was compared to that of the pGEM-T Easy commercial vector. The highest pELMO transformation efficiency was observed for ~500 bp DNA fragments; pELMO vector had higher cloning efficiency for all insert sizes tested. In-house and commercial vector cloned insert reads after sequencing were similar thus highlighting that sequencing primers were designed and localised appropriately. pELMO is thus proposed as a practical alternative for in-house cloning of PCR products in molecular biology laboratories. © 2017, The Author(s). | |
| dc.language | eng | |
| dc.relation | AMB Express, ISSN: 2191-0855, Vol. 7/No. 1 (2017) | |
| dc.relation | https://amb-express.springeropen.com/track/pdf/10.1186/s13568-017-0324-2 | |
| dc.relation | No. 1 | |
| dc.relation | AMB Express | |
| dc.relation | Vol. 7 | |
| dc.rights | info:eu-repo/semantics/openAccess | |
| dc.rights | Abierto (Texto completo) | |
| dc.rights | http://creativecommons.org/licenses/by/4.0/ | |
| dc.source | Ainsa, J.A., Martin, C., Cabeza, M., De la Cruz, F., Mendiola, M.V., Construction of a family of Mycobacterium/Escherichia coli shuttle vectors derived from pAL5000 and pACYC184: their use for cloning an antibiotic-resistance gene from Mycobacterium fortuitum (1996) Gene, 176 (1-2), pp. 23-26. , COI: 1:CAS:528:DyaK28XntVKrtbo%3D, PID: 8918226 | |
| dc.source | instname:Universidad del Rosario | |
| dc.source | reponame:Repositorio Institucional EdocUR | |
| dc.subject | Blunt-Ended | |
| dc.subject | Ccdb Killer Gene | |
| dc.subject | Cloning Vector | |
| dc.subject | Pcr Cloning | |
| dc.subject | Recombinant Dna Technology | |
| dc.title | pELMO, an optimised in-house cloning vector | |
| dc.type | article | |
