Sammanfattning

Pichia stipitis integrates linear homologous DNA fragments mainly ectopically. High rates of randomly occurring integration allow tagging mutagenesis with high efficiency using simply PCR amplificates of suitable selection markers from the P. stipitis genome. Linearization of an autonomously replicating vector caused a distinct increase of the transformation efficiency compared with the circular molecule. Cotransformation of a restriction endonuclease further enhanced the transformation efficiency. This effect was also observed with integrative vector DNA. In most cases vector integration in chromosomal targets did not depend on microhomologies, indicating that restriction-enzyme-mediated integration (REMI) does not play an essential role in P. stipitis. Small deletions were observed at the ends of the integrated vectors and in the target sites. Disruption of the PsKU80 gene increased the frequency of homologous integration considerably but resulted in a remarkable decrease of the transformation efficiency. These results suggest that in P. stipitis the nonhomologous end joining (NHEJ) pathway obviously predominates the homologous recombination pathway of double-strand break repair.

Nyckelord

Pichia stipitis; transformation; tagging mutagenesis; restriction enzyme-mediated integration effect; targeted mutagenesis; nonhomologous end joining

Publicerad i

FEMS Yeast Research
2008, Volym: 8, nummer: 5, sidor: 735-743
Utgivare: BLACKWELL PUBLISHING

SLU författare

• Passoth, Volkmar

  • Institutionen för molekylära vetenskaper, Sveriges lantbruksuniversitet
    

UKÄ forskningsämne

Förnyelsebar bioenergi
Skogsvetenskap


Publikationens identifierare

DOI: https://doi.org/10.1111/j.1567-1364.2008.00383.x

Permanent länk till denna sida (URI)

https://res.slu.se/id/publ/18630