dbCAN-PUL

PUL ID	PUL0590
PubMed	23951303, PLoS One. 2013 Aug 7;8(8):e72285. doi: 10.1371/journal.pone.0072285. eCollection 2013.
Characterization method	qRT-PCR,gene deletion mutant and growth assay,microarray
Genomic accession number	NZ_ABQJ01000017.1
Nucelotide position range	21176-27433
Substrate	maltose,maltodextrin
Loci	EFME1162_RS11430-EFME1162_RS11450
Species	Enterococcus faecium/1352
Degradation or Biosynthesis	degradation

Gene Name	Locus Tag	Protein ID	Gene Position	GenBank Contig Range	EC Number
-	EFME1162_RS11430	WP_002295923.1	0 - 816 (-)	NZ_ABQJ01000017.1:21176-21992	-
-	EFME1162_RS11435	WP_002288156.1	828 - 1680 (-)	NZ_ABQJ01000017.1:22004-22856	-
-	EFME1162_RS11440	WP_002288157.1	1682 - 2984 (-)	NZ_ABQJ01000017.1:22858-24160	-
-	EFME1162_RS11445	WP_002288159.1	3130 - 4390 (-)	NZ_ABQJ01000017.1:24306-25566	-
-	EFME1162_RS11450	WP_002288160.1	4491 - 6258 (-)	NZ_ABQJ01000017.1:25667-27434	-

Cluster number	1
Gene name	Gene position	Gene type	Found by CGCFinder?
-	1 - 816 (-)	CDS	No
-	829 - 1680 (-)	TC: gnl\|TC-DB\|O06991\|3.A.1.1.26	Yes
-	1683 - 2984 (-)	TC: gnl\|TC-DB\|O06990\|3.A.1.1.26	Yes
-	3131 - 4390 (-)	TC: gnl\|TC-DB\|O06989\|3.A.1.1.26	Yes
-	4492 - 6258 (-)	CAZyme: CBM34\|GH13_20	Yes

PUL ID	PUL0590
PubMed	23951303, PLoS One. 2013 Aug 7;8(8):e72285. doi: 10.1371/journal.pone.0072285. eCollection 2013.
Title	A LacI-family regulator activates maltodextrin metabolism of Enterococcus faecium.
Author	Zhang X, Rogers M, Bierschenk D, Bonten MJ, Willems RJ, van Schaik W
Abstract	Enterococcus faecium is a gut commensal of humans and animals. In the intestinal tract, E. faecium will have access to a wide variety of carbohydrates, including maltodextrins and maltose, which are the sugars that result from the enzymatic digestion of starch by host-derived and microbial amylases. In this study, we identified the genetic determinants for maltodextrin utilization of E. faecium E1162. We generated a deletion mutant of the mdxABCD-pulA gene cluster that is homologous to maltodextrin uptake genes in other Gram-positive bacteria, and a deletion mutant of the mdxR gene, which is predicted to encode a LacI family regulator of mdxABCD-pulA. Both mutations impaired growth on maltodextrins but had no effect on the growth on maltose and glucose. Comparative transcriptome analysis showed that eight genes (including mdxABCD-pulA) were expressed at significantly lower levels in the isogenic DeltamdxR mutant strain compared to the parental strain when grown on maltose. Quantitative real-time RT-PCR confirmed the results of transcriptome analysis and showed that the transcription of a putative maltose utilization gene cluster is induced in a semi-defined medium supplemented with maltose but is not regulated by MdxR. Understanding the maltodextrin metabolism of E. faecium could yield novel insights into the underlying mechanisms that contribute to the gut commensal lifestyle of E. faecium.

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