W. van Hartingsveldt scite author profile

The development of a homologous transformation system for Aspergillus niger is described. The system is based on the use of an orotidine-5'-phosphate decarboxylase deficient mutant (pyrG) and a vector, pAB4-1, which contains the functional A. niger pyrG gene as a selection marker. Transformation of the A. niger pyrG mutant with pAB4-1 resulted in the appearance of stable Pyr+ transformants at a frequency of 40 transformants per microgram of DNA. In 90% of these transformants integration had occurred at the resident pyrG locus, resulting either in replacement of the mutant allele by the wild-type allele (60%) or in insertion of one or two copies of the vector (40%). The A. niger pyrG mutant could also be transformed with the vector pDJB2 containing the pyr4 gene of Neurospora crassa, at a frequency of 2 transformants per microgram of DNA. Integration at the resident pyrG locus was not found with this vector. The vector pAB4-1 is also capable of transforming an Aspergillus nidulans pyrG mutant to Pyr+. The pyrG transformation system was used for the introduction of a non-selectable gene into A. niger.

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**The Aspergillus nigerGCN4 homologue, cpcA, is transcriptionally regulated and encodes an unusual leucine zipper**

Wanke

Eckert

Albrecht

et al. 1997

Molecular Microbiology

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SummaryThe general control transcriptional regulator gene cpcA of Aspergillus niger was cloned by complementation of a Saccharomyces cerevisiae ⌬gcn4 mutant strain. The encoded protein conferred resistance to amino acid analogues when expressed in yeast. Disruption of cpcA in A. niger resulted in a strain which is sensitive towards 3-aminotriazole and fails to respond to amino acid starvation. cpcA encodes a transcript of Ϸ2400 nucleotides in length that includes a 5Ј leader region of 900 nucleotides. The 5Ј leader region contains two small open reading frames, suggesting translational control of gene expression. Steadystate mRNA levels of cpcA increase by a factor of three upon amino acid starvation. The coding region of cpcA is interrupted by a 57 bp intron and the deduced amino acid sequence displays an Ϸ30% overall identity to yeast GCN4p and Neurospora crassa cpc1p. Critical amino acid residues of the transcriptional activation domains of GCN4p are conserved in cpcAp. The basic DNA-binding domain shows up to 70% amino acid sequence identity to other basic zipper (bZIP)-type transcriptional activators. cpcAp binds specifically to a GCN4p recognition element in gel retardation experiments. The C-terminal dimerization domain encodes a leucine zipper with only a single leucine residue.

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Cloning, characterization and overexpression of the phytase-encoding gene (phyA) of Aspergillus niger

Hartingsveldt¹,

Zeijl²,

Harteveld³

et al. 1993

Gene

159

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Cloning of the nitrate - nitrite reductase gene cluster of Penicillium chrysogenum and use of the niaD gene as a homologous selection marker

Gouka¹,

Hartingsveldt²,

Bovenberg

et al. 1991

Journal of Biotechnology

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Enantioselective oxidation of secondary alcohols at a quinohaemoprotein alcohol dehydrogenase electrode

Somers

Stigter

Hartingsveldt

et al. 1998

Appl Biochem Biotechnol

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