Schema for D. hydei (DhydRS2) Chain - D. hydei (May 2019 (The University of Chicago/DhydRS2)) Chained Alignments

JavaScript is disabled in your web browser

You must have JavaScript enabled in your web browser to use the Genome Browser

Schema for D. hydei (DhydRS2) Chain - D. hydei (May 2019 (The University of Chicago/DhydRS2)) Chained Alignments

Database: DhydGB1 Primary Table: chainDhydRS2 Row Count: 17,404 Data last updated: 2022-10-20

field	example	SQL type	info
`bin`	585	`smallint(5) unsigned`	range
`score`	48890	`double`	range
`tName`	NWQH01000001	`varchar(255)`	values
`tSize`	3368585	`int(10) unsigned`	range
`tStart`	0	`int(10) unsigned`	range
`tEnd`	898	`int(10) unsigned`	range
`qName`	QMEQ02000074	`varchar(255)`	values
`qSize`	825448	`int(10) unsigned`	range
`qStrand`	+	`char(1)`	values
`qStart`	4616	`int(10) unsigned`	range
`qEnd`	5514	`int(10) unsigned`	range
`id`	18112	`int(10) unsigned`	range

Sample Rows

bin	score	tName	tSize	tStart	tEnd	qName	qSize	qStrand	qStart	qEnd	id
585	48890	NWQH01000001	3368585	0	898	QMEQ02000074	825448	+	4616	5514	18112
585	25464	NWQH01000001	3368585	0	439	QMEQ02000074	825448	+	3699	4137	39574
585	704248	NWQH01000001	3368585	0	17194	QMEQ02000065	1382317	+	123399	138270	603
585	13298	NWQH01000001	3368585	0	234	QMEQ02000074	825448	+	5993	6227	67057
585	18363	NWQH01000001	3368585	0	282	QMEQ02000040	5146216	+	10431	10713	53109
73	72290450	NWQH01000001	3368585	0	805205	QMEQ02000074	825448	+	2213	825448	39
585	19272	NWQH01000001	3368585	0	366	QMEQ02000074	825448	+	3284	3640	50965
585	22021	NWQH01000001	3368585	0	439	QMEQ02000074	825448	+	6452	6861	45436
585	223311	NWQH01000001	3368585	0	3861	QMEQ02000074	825448	+	2672	6227	2102
585	49655	NWQH01000001	3368585	0	894	QMEQ02000207	1857246	+	27776	28669	17757

Note: all start coordinates in our database are 0-based, not 1-based. See explanation here.

D. hydei (DhydRS2) Chain (chainDhydRS2) Track Description


	Description This track shows D. hydei/D. hydei genomic alignments using a gap scoring system that allows longer gaps than traditional affine gap scoring systems. It can also tolerate gaps in both D. hydei and D. hydei simultaneously. These "double-sided" gaps can be caused by local inversions and overlapping deletions in both species. The D. hydei sequence is from the May 2019 (The University of Chicago/DhydRS2) (DhydRS2) assembly. The chain track displays boxes joined together by either single or double lines. The boxes represent aligning regions. Single lines indicate gaps that are largely due to a deletion in the D. hydei assembly or an insertion in the D. hydei assembly. Double lines represent more complex gaps that involve substantial sequence in both species. This may result from inversions, overlapping deletions, an abundance of local mutation, or an unsequenced gap in one species. In cases where there are multiple chains over a particular portion of the D. hydei genome, chains with single-lined gaps are often due to processed pseudogenes, while chains with double-lined gaps are more often due to paralogs and unprocessed pseudogenes. In the "pack" and "full" display modes, the individual feature names indicate the chromosome, strand, and location (in thousands) of the match for each matching alignment. Display Conventions and Configuration By default, the chains to chromosome-based assemblies are colored based on which chromosome they map to in the aligning organism. To turn off the coloring, check the "off" button next to: Color track based on chromosome. To display only the chains of one chromosome in the aligning organism, enter the name of that chromosome (e.g. chr4) in box next to: Filter by chromosome. Methods Transposons that have been inserted since the D. hydei/D. hydei split were removed, and the resulting abbreviated genomes were aligned with blastz. The transposons were then put back into the alignments. The resulting alignments were converted into axt format and the resulting axts fed into axtChain. AxtChain organizes all the alignments between a single D. hydei and a single D. hydei chromosome into a group and makes a kd-tree out of all the gapless subsections (blocks) of the alignments. Next, maximally scoring chains of these blocks were found by running a dynamic program over the kd-tree. Chains scoring below a threshold were discarded; the remaining chains are displayed here. Credits Blastz was developed at Pennsylvania State University by Minmei Hou, Scott Schwartz, Zheng Zhang, and Webb Miller with advice from Ross Hardison. Lineage-specific repeats were identified by Arian Smit and his program RepeatMasker. The axtChain program was developed at the University of California at Santa Cruz by Jim Kent with advice from Webb Miller and David Haussler. The browser display and database storage of the chains were generated by Robert Baertsch and Jim Kent. References Chiaromonte, F., Yap, V.B., Miller, W. Scoring pairwise genomic sequence alignments. Pac Symp Biocomput 2002, 115-26 (2002). Kent, W.J., Baertsch, R., Hinrichs, A., Miller, W., and Haussler, D. Evolution's cauldron: Duplication, deletion, and rearrangement in the mouse and human genomes. Proc Natl Acad Sci USA 100(20), 11484-11489 (2003). Schwartz, S., Kent, W.J., Smit, A., Zhang, Z., Baertsch, R., Hardison, R., Haussler, D., and Miller, W. Human-Mouse Alignments with BLASTZ. Genome Res. 13(1), 103-7 (2003).