dbCAN-PUL

PUL ID	PUL0246
PubMed	24333485, J Mol Biol. 2014 Apr 3;426(7):1469-82. doi: 10.1016/j.jmb.2013.12.006. Epub 2013 Dec 12.
Characterization method	enzyme activity assay,gene deletion mutant and growth assay,Western Blot
Genomic accession number	AAZZ01000003.1
Nucelotide position range	96120-112614
Substrate	fucose
Loci	CGSSp3BS71_10393-CGSSp3BS71_10443
Species	Streptococcus pneumoniae/1313
Degradation or Biosynthesis	degradation

Gene Name	Locus Tag	Protein ID	Gene Position	GenBank Contig Range	EC Number
-	CGSSp3BS71_10393	EDK74347.1	0 - 1767 (-)	AAZZ01000003.1:96120-97887	-
-	CGSSp3BS71_10398	EDK74348.1	1779 - 2508 (-)	AAZZ01000003.1:97899-98628	-
-	CGSSp3BS71_10403	EDK74349.1	2522 - 5540 (-)	AAZZ01000003.1:98642-101660	-
-	CGSSp3BS71_10408	EDK74350.1	5550 - 7767 (-)	AAZZ01000003.1:101670-103887	-
-	CGSSp3BS71_10413	EDK74351.1	8006 - 9659 (-)	AAZZ01000003.1:104126-105779	-
-	CGSSp3BS71_10418	EDK74352.1	9664 - 10972 (-)	AAZZ01000003.1:105784-107092	-
-	CGSSp3BS71_10423	EDK74353.1	10981 - 11827 (-)	AAZZ01000003.1:107101-107947	-
-	CGSSp3BS71_10428	EDK74354.1	11823 - 12753 (-)	AAZZ01000003.1:107943-108873	-
-	CGSSp3BS71_10433	EDK74355.1	12839 - 14132 (-)	AAZZ01000003.1:108959-110252	-
-	CGSSp3BS71_10438	EDK74356.1	14160 - 15564 (-)	AAZZ01000003.1:110280-111684	-
-	CGSSp3BS71_10443	EDK74357.1	15739 - 16495 (+)	AAZZ01000003.1:111859-112615	-

Cluster number	1
Gene name	Gene position	Gene type	Found by CGCFinder?
-	1 - 1767 (-)	CDS	No
-	1780 - 2508 (-)	CDS	No
-	2523 - 5540 (-)	CAZyme: GH98\|CBM51	Yes
-	5551 - 7767 (-)	CAZyme: GH36	Yes
-	8007 - 9659 (-)	CAZyme: GH36	Yes
-	9665 - 10972 (-)	CAZyme: GH29	Yes
-	10982 - 11827 (-)	TC: gnl\|TC-DB\|A5LBQ4\|3.A.1.1.47	Yes
-	11824 - 12753 (-)	TC: gnl\|TC-DB\|A5LBQ5\|3.A.1.1.47	Yes
-	12840 - 14132 (-)	TC: gnl\|TC-DB\|A5LBQ6\|3.A.1.1.47	Yes
-	14161 - 15564 (-)	CDS	No
-	15740 - 16495 (+)	TF: DBD-Pfam\|HTH_DeoR,DBD-SUPERFAMILY\|0043758	No

PUL ID	PUL0246
PubMed	24333485, J Mol Biol. 2014 Apr 3;426(7):1469-82. doi: 10.1016/j.jmb.2013.12.006. Epub 2013 Dec 12.
Title	Structural and functional analysis of fucose-processing enzymes from Streptococcus pneumoniae.
Author	Higgins MA, Suits MD, Marsters C, Boraston AB
Abstract	Fucose metabolism pathways are present in many bacterial species and typically contain the central fucose-processing enzymes fucose isomerase (FcsI), fuculose kinase (FcsK), and fuculose-1-phosphate aldolase (FcsA). Fucose initially undergoes isomerization by FcsI producing fuculose, which is then phosphorylated by FcsK. FcsA cleaves the fuculose-1-phosphate product into lactaldehyde and dihydroxyacetone phosphate, which can be incorporated into central metabolism allowing the bacterium to use fucose as an energy source. Streptococcus pneumoniae has fucose-processing operons containing homologs of FcsI, FcsK, and FcsA; however, this bacterium appears unable to utilize fucose as an energy source. To investigate this contradiction, we performed biochemical and structural studies of the S. pneumoniae fucose-processing enzymes SpFcsI, SpFcsK, and SpFcsA. These enzymes are demonstrated to act in a sequential manner to ultimately produce dihydroxyacetone phosphate and have structural features entirely consistent with their observed biochemical activities. Analogous to the regulation of the Escherichia coli fucose utilization operon, fuculose-1-phosphate appears to act as an inducing molecule for activation of the S. pneumoniae fucose operon. Despite our evidence that S. pneumoniae appears to have the appropriate regulatory and biochemical machinery for fucose metabolism, we confirmed the inability of the S. pneumoniae TIGR4 strain to grow on fucose or on the H-disaccharide, which is the probable substrate of the transporter for the pathway. On the basis of these observations, we postulate that the S. pneumoniae fucose-processing pathway has a non-metabolic role in the interaction of this bacterium with its human host.

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