dbCAN-PUL

PUL ID	PUL0268
PubMed	23793634, Appl Environ Microbiol. 2013 Sep;79(17):5151-8. doi: 10.1128/AEM.01506-13. Epub 2013 Jun 21.
Characterization method	Northern Blot,promoter assay
Genomic accession number	BA000043.1
Nucelotide position range	726823-732934
Substrate	starch
Loci	GK0704-GK0708
Species	Geobacillus kaustophilus/1462
Degradation or Biosynthesis	degradation

Gene Name	Locus Tag	Protein ID	Gene Position	GenBank Contig Range	EC Number
-	GK0704	BAD74989.1	0 - 1275 (+)	BA000043.1:726823-728098	-
-	GK0705	BAD74990.1	1344 - 2625 (+)	BA000043.1:728167-729448	-
-	GK0706	BAD74991.1	2624 - 3467 (+)	BA000043.1:729447-730290	-
-	GK0707	BAD74992.1	3532 - 5074 (+)	BA000043.1:730355-731897	3.2.1.1
-	GK0708	BAD74993.1	5092 - 6112 (+)	BA000043.1:731915-732935	-

Cluster number	1
Gene name	Gene position	Gene type	Found by CGCFinder?
-	1 - 1275 (+)	TC: gnl\|TC-DB\|O07009\|3.A.1.1.2	Yes
-	1345 - 2625 (+)	TC: gnl\|TC-DB\|O32261\|3.A.1.1.2	Yes
-	2625 - 3467 (+)	TC: gnl\|TC-DB\|O07011\|3.A.1.1.2	Yes
-	3533 - 5074 (+)	CAZyme: GH13_1\|GH13	Yes
-	5093 - 6112 (+)	STP: STP\|LacI,STP\|Peripla_BP_3	No

PUL ID	PUL0268
PubMed	23793634, Appl Environ Microbiol. 2013 Sep;79(17):5151-8. doi: 10.1128/AEM.01506-13. Epub 2013 Jun 21.
Title	Polysaccharide-degrading thermophiles generated by heterologous gene expression in Geobacillus kaustophilus HTA426.
Author	Suzuki H, Yoshida K, Ohshima T
Abstract	Thermophiles have important advantages over mesophiles as host organisms for high-temperature bioprocesses, functional production of thermostable enzymes, and efficient expression of enzymatic activities in vivo. To capitalize on these advantages of thermophiles, we describe here a new inducible gene expression system in the thermophile Geobacillus kaustophilus HTA426. Six promoter regions in the HTA426 genome were identified and analyzed for expression profiles using beta-galactosidase reporter assay. This analysis identified a promoter region upstream of a putative amylose-metabolizing gene cluster that directed high-level expression of the reporter gene. The expression was >280-fold that without a promoter and was further enhanced 12-fold by maltose addition. In association with a multicopy plasmid, this promoter region was used to express heterologous genes. Several genes, including a gene whose product was insoluble when expressed in Escherichia coli, were successfully expressed as soluble proteins, with yields of 0.16 to 59 mg/liter, and conferred new functions to G. kaustophilus strains. Remarkably, cellulase and alpha-amylase genes conferred the ability to degrade cellulose paper and insoluble starch at high temperatures, respectively, generating thermophiles with the potential to degrade plant biomass. Our results demonstrate that this novel expression system expands the potential applications of G. kaustophilus.

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