Latest revision as of 11:04, 21 December 2011

Instructions for curators

With the move to the new paper editor, the instructions on this page are now obsolete. --kjy 18:03, 29 July 2010 (UTC)

Feature Requests

New First Pass Curator form

"flagged" = WBPapers that have been flagged for that particular data type but not curated yet or not assessed for curation status yet; "flagged-done" = WBPapers that have been flagged and curated. These papers can be used as a source for verified curation flag examples. Click the "?" to find out more about the data type.

Automation status	Paper Section	Data type	Old fp curation form name	PGdb name	Description for author	Curator Flagged	Notes about field
		SPECIES:
	materials and methods	C. elegans default checked.	new field	celegans	Uncheck if you are NOT reporting data for C. elegans.
	materials and methods	C. elegans other than Bristol	new field	cnonbristol	Check if data for C. elegans natural isolates other than N2 (Bristol) are reported.e.g. Hawaiian, CB4855, CB4852, CB4507, LSJ1, etc.
	materials and methods	Nematodes other than C. elegans	nonntwo	nematode	Check if data is reported for any species other than C. elegans, e.g., C. briggsae, Pristionchus pacificus, Brugia malayi, etc.
	materials and methods	Non-nematode species	new field	nonnematode	Check if data is reported for any non-nematode species.
		GENE IDENTIFICATION AND MAPPING:
		Genes studied in this paper		genestudied	List any gene for which you report experimental results; do not include genetic markers.		Big text box, auto-opened.
in progress		Newly cloned gene (flagged-done)	Gene Symbol	genesymbol	Check if your paper reports a new symbol for a known locus or the name of a newly defined locus.	genenames@wormbase.org, vanauken@its.caltech.edu
in progress		Newly created allele	Extract allele	extvariation	Check if your paper reports the identification of any allele that doesn't exist in WormBase already.
		Genetic mapping data (flagged)	mapping data	mappingdata	Check if your paper contains 3-factor interval mapping data, i.e., genetic data only. Include Df or Dp data, but no SNP interval mapping.	genenames@wormbase.org
		GENE FUNCTION:
		Mutant, RNAi, overexpression, or chemical-based phenotypes:				PLEASE SPECIFY DATA TYPE.
DONE		Phenotype analysis (flagged-done)	Mutant Phenotype	newmutant	Check if your paper reports phenotype due to mutation or overexpression analysis.	remove-emsch@its.caletch.edu, garys@its.caltech.edu, jolenef@its.caltech.edu
DONE		Small-scale RNAi (less than 100 experiments reported) (flagged-done)	RNAi	rnai	Check if your paper reports gene knockdown phenotypes for less than 100 individual RNAi experiments.	garys@its.caltech.edu
DONE will be part of small scale RNAi pipeline		Large-scale RNAi (less than 100 experiments reported) (flagged-done)	Large-Scale RNAi	lsrnai	Check if your paper reports gene knockdown phenotypes for more than 100 individual RNAi experiments.	raymond@its.caltech.edu
DONE through phenotype analysis		Overexpression phenotype (flagged)	Overexpression	overexpr	Check if your paper reports an abnormal phenotype based on the overexpression of a gene or gene construct. E.g., ""...constitutively activated SCD-2(neu*) receptor caused 100% of animals to arrest in the first larval stage (L1)..."	remove-emsch@its.caletch.edu, garys@its.caltech.edu, jolenef@its.caltech.edu
in progress	materials and methods; results	Chemicals (flagged)	Chemicals	chemicals	Check if the effects of small molecules, chemicals, or drugs were studied on worms. E.g., paraquat, butanone, benzaldehyde, aldicarb, etc. Mutagens used for the generation of mutant in genetic screens do not need to be indicated.
		Mosaic analysis (flagged-done)	Mosaic analysis	mosaic	Check if your paper reports cell specific gene function based on mosaic analysis, e.g. extra-chromosomal transgene loss in a particular cell lineage leads to loss of mutant rescue, etc.	raymond@its.caltech.edu
		Tissue or cell site of action (flagged-done)	Site of action	siteaction	Check if your paper reports anatomy-specific function for a gene.	raymond@its.caltech.edu
		Time of action	new field	timeaction	Check if your paper reports a temporal requirement for gene function, that is, if gene activity was assayed, for example, through temperature-shift experiments.	raymond@its.caltech.edu
		Molecular function of a gene product(flagged-done)	Gene function	genefunc	Check if your paper discusses a new function for a known or newly defined gene.	remove emsch@its.caletch.edu
in progress		Homolog of a human disease-associated gene.(flagged)	Human Disease	humdis	Check if genes discussed in your paper are a homolog/ortholog of a human disease-related gene or if your study models some aspect of a human disease.	ranjana@its.caltech.edu
		INTERACTIONS:
		Genetic interactions (flagged-done)	Gene interactions	geneint	Check if your paper reports the analysis of more than one gene at a time, e.g., double, triple, etc. mutants, including experiments where RNAi was concurrent with other RNAi-treatments or mutations.	remove emsch@its.caletch.edu
	materials and methods (tools); results	Functional complementation (flagged)	Functional Complementation	funccomp	Check if your paper reports functional redundancy between separate genes, e.g. the rescue of gen-A by overexpression of gen-B or any other extragenic sequence.
		Gene product interactions (flagged-done)	Gene product interaction	geneprod	Check if your paper reports data on protein-protein, RNA-protein, DNA-protein or Y2H interactions, etc.	remove emsch@its.caletch.edu
		REGULATION OF GENE EXPRESSION:
some SVM (not great)		New expression pattern for a gene (flagged-done)	expression pattern data	otherexpr	Check if your paper reports new temporal or spatial (e.g., tissue, subcellular, etc.) data on the pattern of expression of any gene in a wild-type background. You can include: reporter gene analysis, antibody staining, In situ hybridization, RT-PCR, Western or Northern blot data.	wchen@its.caltech.edu, vanauken@its.caltech.edu
some SVM (not great)		Alterations in gene expression by genetic or other treatment (flagged-done)	Gene regulation on expression level	genereg	Check if your paper reports changes or lack of changes in gene expression levels or patterns due to genetic, chemical, temperature, or any other experimental treatment.	xdwang@its.caltech.edu
		Regulatory sequence features (flagged)	Sequence features	seqfeat	Check if your paper reports any gene expression regulatory elements, e.g., DNA/RNA elements required for gene expression, promoters, introns, UTR's, DNA binding sites, etc.	xdwang@its.caltech.edu, worm-bug@sanger.ac.uk, stlouis@wormbase.org
		Position frequency matrix (PFM) or Position weight matrix (PWM)	new field	matrices	Check if your paper reports PFMs or PWMs, which are typically used to define regulatory sites in genomic DNA (e.g., bound by transcription factors) or mRNA (e.g., bound by translational factors or miRNA). PFMs define simple nucleotide frequencies, while PWMs are scaled logarithmically against a background frequency.	xdwang@its.caltech.edu, remove- emsch@its.caletch.edu
		Microarray(flagged-done)	Microarray	microarray	Check if your paper reports any microarray data.	wchen@its.caltech.edu
		PROTEIN FUNCTION AND STRUCTURE:
Kimberly said to remove this	materials and methods; results	Protein analysis in vitro(flagged)	in vitro Protein analysis	invitro	Check if your paper reports any in vitro protein analysis such as kinase assays, agonist pharmacological studies, in vitro reconstitution studies, etc.
	materials and methods; results	Domain analysis	new field	domanal (populated with information previously in "structureinformation")	Check if your paper reports on a function of a particular domain within a protein.
	materials and methods; results	Covalent modification (flagged)	Covalent modification	covalent	Check if your paper reports on post-translational modifications as assayed by mutagenesis or in vitro analysis
	materials and methods; results	Structural information(flagged)	Structure information	structinfo	Check if your paper reports NMR or X-ray crystallographic information.		besides structure info (e.g. x-ray crystallography data) Andrei also includes structure-function data (e.g. mutation at Ser-321 compromises folding, binding, etc.)
		Mass spectrometry (flagged-done)	Mass Spec	massspec	Check if your paper reports data from any mass spec analysis; keywords: mass spectrometry, peptide, (and any one of the following:) MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix.	gw3@ebi.ac.uk, worm-bug@sanger.ac.uk	From Gary "...only interested in papers that report the peptide sequences that the mass-spec fragments match. These peptides are usually created by one of the programs: MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix. So, the Description field should be: Keywords: mass spectrometry, peptide, (and any one of the following:) MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix
		REAGENTS:
DONE		C. elegans antibodies (flagged-done)	Extract Antibody	antibody	Check if your paper reports the use of new or known antibodies created by your lab or someone else's lab; do not check this box if antibodies were commercially bought.	wchen@its.caltech.edu
DONE		Integrated transgenes (flagged-done)	Transgene	transgene	Check if integrated transgenes were used in this paper. If the transgene does not have a canonical name, please list it in the "Add Information text area"	wchen@its.caltech.edu
		Transgenes used as tissue markers	Marker	marker	Check if reporters (integrated transgenes) were used to mark certain tissues, subcellular structures, or life stages, etc. as a reference point to assay gene function or location.	wchen@its.caltech.edu, vanauken@its.caltech.edu
		GENOME SEQUENCE DATA:
		Gene structure correction (flagged)	Sanger Gene Structure Correction and St. Louis Gene Structure Correction	structcorr (this use to be two different fields)	Check if your paper reports a gene structure that is different from the one in WormBase, e.g., different splice-site, SL1 instead of SL2, etc.	worm-bug@sanger.ac.uk, wormticket@watson.wustl.edu	the authors may or may not state explicitly that let's say there is a novel exon. if i see a gene studied in some detail (e.g. new gene was cloned or gene structure is drawn in fig.), than i check amino acid length for the protein with the data in WB, and i will eyeball the diagrams of gene structures to see if there are obvious diffs. these are quick checks but they catch an occasional gene structure change not listed in the text.
		Sequencing mutant alleles (flagged)	Sequence change	seqchange	Check if your paper reports new sequence data for any mutation.	genenames@wormbase.org
		New SNPs (flagged)	Extract New SNP	newsnp	Check if your paper reports a SNP that does not already exist in WormBase.	dblasiar@watson.wustl.edu, tbieri@watson.wustl.edu
		CELL DATA:
		Ablation data (flagged-done)	Ablation data	ablationdata	Check if your paper reports data from an assay involving any cell or anatomical unit being ablated by laser or by other means (e.g., by expressing a cell-toxic protein).	raymond@its.caltech.edu
		Cell function (flagged-done)	Cell function	cellfunc	Check if your paper reports a function for any anatomical part (e.g., cell, tissue, etc.), which has not been indicated elsewhere on this form.	raymond@its.caltech.edu
		IN SILICO DATA:
		Phylogenetic data	new field	phylogenetic	Check if your paper reports any phylogenetic analysis.
		Other bioinformatics analysis	new field	othersilico	Check if your paper reports any bioinformatic data not indicated anywhere else on this form.
		OTHER:
		Supplemental materials (flagged-done)	Supplemental material	supplemental	Check if your paper has supplemental material.	qwang@its.caltech.edu
		NONE of the aforementioned data types are in this research article (flagged)	Comment	nocuratable	Check if none of the above pertains to your paper. Feel free to list the data type most pertinent to your research paper in the "Add information" text area.
		Any feedback? Please feel free to give us feedback for this form or for any other topic pertinent to how we can better extract data from your paper.	new field	comment	Comments from all authors and curators are accessible through the "Comment" button at the bottom of the page.	kyook@caltech.edu, vanauken@caltech.edu

--kjy 17:56, 29 July 2010 (UTC)

@@ Line 1: / Line 1: @@
 [[http://www.wormbase.org/wiki/index.php/How_to_FirstPass back]]
+----
+=[[Instructions for curators]]=
+With the move to the new paper editor, the instructions on this page are now obsolete. --kjy 18:03, 29 July 2010 (UTC)
+=[[Feature Requests]]=
+----
 =New First Pass Curator form=
 ''"flagged" = WBPapers that have been flagged for that particular data type but not curated yet or not assessed for curation status yet; "flagged-done" = WBPapers that have been flagged and curated. These papers can be used as a source for verified curation flag examples.''
+'''Click the "?" to find out more about the data type.'''
 {|| border="1" cellpadding="2"
 | width="50"align="center" style="background:#f0f0f0;"|'''Automation status'''
-| align="center" style="background:#f0f0f0;"|'''Data type Section'''
+| align="center" style="background:#f0f0f0;"|'''Paper Section'''
 | align="center" style="background:#f0f0f0;"|'''Data type'''
-| align="center" style="background:#f0f0f0;"|'''''Old curation form name''; PGdb name'''
+| align="center" style="background:#f0f0f0;"|'''Old fp curation form name'''
+| align="center" style="background:#f0f0f0;"|'''PGdb name'''
 | align="center" style="background:#f0f0f0;"|'''Description for author'''
 | align="center" style="background:#f0f0f0;"|'''Curator Flagged'''
+| align="center" style="background:#f0f0f0;"|'''Notes about field'''
 |-
-|||GENE IDENTIFICATION AND MAPPING:
+|||||colspan="6"|SPECIES:
 |-
-|||||'''''C. elegans'''''|| '''new field''' = celegans||Please indicate if ''C. elegans'' isolates other than Bristol are discussed in this paper|||
+|||materials and methods||'''''C. elegans'''''  ''default checked.''||'''new field'''||'''celegans'''||'''Uncheck''' if you are NOT reporting data for ''C. elegans''.||||
 |-
-|||||'''Nematodes other than ''C. elegans'''''||'''new field''' = nematodes||Please indicate if data is presented for any species other than ''C. elegans'', e.g., ''C. briggsae'', ''Pristionchus pacificus'', ''Brugia malayi'', etc.||
+|||materials and methods||'''''C. elegans'' other than Bristol'''|| '''new field'''|| cnonbristol ||Check if data for ''C. elegans'' natural isolates other than N2 (Bristol) are reported.''e.g. Hawaiian, CB4855, CB4852, CB4507, LSJ1, etc.''||||
 |-
-|||||'''Newly cloned gene''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=genesymbol (flagged-done)]||''Gene Symbol'' ; genesymbol ||Please indicate if your paper presents a new symbol for a known locus or the name of a newly defined locus.||genenames@wormbase.org, vanauken@its.caltech.edu
+|||materials and methods||'''Nematodes other than ''C. elegans'''''||nonntwo||nematode||Check if data is reported for any species other than ''C. elegans'', e.g., ''C. briggsae'', ''Pristionchus pacificus'', ''Brugia malayi'', etc. ||||
 |-
-|in progress||||'''Newly created allele'''||''Extract allele'' ; extractedvariation||Please indicate if your paper reports the identification of any new alleles.||
+|||materials and methods||'''Non-nematode species'''||'''new field'''||nonnematode||Check if data is reported for any non-nematode species.||||
 |-
-|||||'''Genetic mapping data''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=mappingdata (flagged)]||''mapping data'' ; mappingdata||Please indicated if your paper contains 3-factor interval mapping data, i.e., genetic data only, including with Df or Dp data but no SNP interval mapping.||genenames@wormbase.org
+|||||colspan="6"|GENE IDENTIFICATION AND MAPPING:
 |-
-|||GENE FUNCTION:
+|||||'''Genes studied in this paper'''||||genestudied||List any gene for which you report experimental results; do not include genetic markers.|||| '''Big text box, auto-opened.'''
 |-
-|||||'''Gene function''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=genefunction (flagged-done)]||''Gene function'' ; genefunction||Please indicate if your paper discusses a new function for a known gene or a newly defined gene.||emsch@its.caltech.edu
+|in progress||||'''Newly cloned gene''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=genesymbol (flagged-done)]||''Gene Symbol''|| genesymbol ||Check  if your paper reports a new symbol for a known locus or the name of a newly defined locus.||genenames@wormbase.org, vanauken@its.caltech.edu ||
 |-
-|in progress||||'''Homolog of a human disease-associated gene''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=humandiseases (flagged)]||''Human Disease'' ; humandiseases ||Please indicate if genes discussed in your paper are a homolog/ortholog of a human disease gene.
+|in progress||||'''Newly created allele'''||''Extract allele''||extvariation||Check if your paper reports the identification of any allele that doesn't exist in WormBase already.||||
-||ranjana@its.caltech.edu
 |-
-|||Phenotype Analysis based on:
+|||||'''Genetic mapping data''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=mappingdata (flagged)]||''mapping data''||mappingdata||Check if your paper contains 3-factor interval mapping data, i.e., genetic data only. Include Df or Dp data, but no SNP interval mapping.||genenames@wormbase.org ||
 |-
-|||||'''Allele analysis''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=newmutant (flagged-done)]|| ''Mutant Phenotype''; newmutant ||Please indicate if any phenotype is reported for a mutant variation. ||emsch@its.caltech.edu, garys@its.caltech.edu, jolenef@its.caltech.edu
+|||||colspan="6"|GENE FUNCTION:
 |-
-||in progress||||'''Small-scale RNAi''' (less than 100 experiments reported) [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=rnai (flagged-done)]||''RNAi'' ; rnai||Please indicate if your paper reports gene knockdown phenotypes for less than 100 individual RNAi experiments.||garys@its.caltech.edu
+|||||colspan="4"|'''Mutant, RNAi, overexpression, or chemical-based phenotypes''':||colspan="2"|'''PLEASE SPECIFY DATA TYPE.'''
 |-
-||||||'''Large-scale RNAi''' (less than 100 experiments reported) [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=lsrnai (flagged-done)]||''Large-Scale RNAi'' ; lsrnai||Please indicate if your paper reports gene knockdown phenotypes for more than 100 individual RNAi experiments.||raymond@its.caltech.edu
+|'''DONE'''||||'''Phenotype analysis''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=newmutant (flagged-done)]|| ''Mutant Phenotype''|| newmutant ||Check if your paper reports phenotype due to mutation or overexpression analysis. ||remove-'''emsch@its.caletch.edu''', garys@its.caltech.edu, jolenef@its.caltech.edu ||
 |-
-|||||'''Overexpression''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=overexpression (flagged)]||''Overexpression'' ; overexpression||Please indicated if your paper reports an abnormal phenotype based on the overexpression of a gene or gene construct. E.g., ""...constitutively activated SCD-2(neu*) receptor caused 100% of animals to arrest in the first larval stage (L1)..." ||emsch@its.caltech.edu, garys@its.caltech.edu
+|'''DONE'''||||'''Small-scale RNAi''' (less than 100 experiments reported) [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=rnai (flagged-done)]||''RNAi''|| rnai||Check if your paper reports gene knockdown phenotypes for less than 100 individual RNAi experiments.||garys@its.caltech.edu||
 |-
-|in progress||||'''Chemicals''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=chemicals (flagged)]||''Chemicals'' ; chemicals ||Please indicate if the effects of small molecules, chemicals, or drugs were studied on worms. E.g., paraquat, butanone, benzaldehyde, aldicarb, etc. Mutagens used for the generation of mutant in genetic screens do not need to be indicated.|||
+|'''DONE''' ''will be part of small scale RNAi pipeline''||||'''Large-scale RNAi''' (less than 100 experiments reported) [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=lsrnai (flagged-done)]||''Large-Scale RNAi''|| lsrnai||Check if your paper reports gene knockdown phenotypes for more than 100 individual RNAi experiments.||raymond@its.caltech.edu||
 |-
-|||INTERACTIONS:
+|'''DONE''' through phenotype analysis||||'''Overexpression phenotype''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=overexpression (flagged)]||''Overexpression''|| overexpr||Check if your paper reports an abnormal phenotype based on the overexpression of a gene or gene construct. E.g., ""...constitutively activated SCD-2(neu*) receptor caused 100% of animals to arrest in the first larval stage (L1)..." ||remove-'''emsch@its.caletch.edu''', garys@its.caltech.edu, jolenef@its.caltech.edu||
 |-
+|in progress||materials and methods; results||'''Chemicals''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=chemicals (flagged)]||''Chemicals''|| chemicals ||Check if the effects of small molecules, chemicals, or drugs were studied on worms. E.g., paraquat, butanone, benzaldehyde, aldicarb, etc. Mutagens used for the generation of mutant in genetic screens do not need to be indicated.||||
 |-
-|||GENE EXPRESSION AND FUNCTION:
+|||||'''Mosaic analysis''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=mosaic (flagged-done)]||''Mosaic analysis''||mosaic ||Check if your paper reports cell specific gene function based on mosaic analysis, e.g. extra-chromosomal transgene loss in a particular cell lineage leads to loss of mutant rescue, etc. ||raymond@its.caltech.edu ||
 |-
-|||||'''New expression pattern for a gene''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=expression (flagged-done)]||''expression pattern data'' ; otherexpression ||Please indicate if your paper reports new temporal or spatial (e.g. tissue, subcellular, etc) data on the pattern of expression of any gene in a wild-type background. You can include:  reporter gene analysis, antibody staining, ''In situ'' hybridization, RT-PCR, Western or Northern blot data.||wchen@its.caltech.edu, vanauken@its.caltech.edu
+|||||'''Tissue or cell site of action''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=site (flagged-done)]||''Site of action''|| siteaction ||Check if your paper reports anatomy-specific function for a gene.||raymond@its.caltech.edu ||
 |-
-|||Tools used for obtaining an expression pattern for a new gene:
+|||||'''Time of action'''||'''new field''' || timeaction||Check if your paper reports a temporal requirement for gene function, that is, if gene activity was assayed, for example, through temperature-shift experiments.||raymond@its.caltech.edu||
 |-
-|in progress||||'''''C. elegans'' antibodies''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=antibody (flagged-done)]||''Extract Antibody'' ; antibodies ||Please indicate if your paper reports the use of new or used antibodies created by your lab or someone else's lab; do not check this box if antibodies used were commercially bought.||wchen@its.caltech.edu
+|||||'''Molecular function of a gene product'''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=genefunction (flagged-done)]||''Gene function''||genefunc||Check if your paper discusses a new function for a known or newly defined gene.||remove '''emsch@its.caletch.edu''' ||
 |-
-|'''DONE'''||||'''Integrated transgenes''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=transgene (flagged-done)] ||''Transgene'' ; transgene||Please indicate if integrated transgenes are used in this paper. If the transgene does not have a canonical name, please list it in the "Add Information text area" ||wchen@its.caltech.edu
+|in progress||||'''Homolog of a human disease-associated gene.'''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=humandiseases (flagged)]||''Human Disease''|| humdis ||Check if genes discussed in your paper are a homolog/ortholog of a human disease-related gene or if your study models some aspect of a human disease.||ranjana@its.caltech.edu ||
 |-
-|||||'''Cell/Tissue reporters''' ||''Marker'' ; marker||Please indicate if reporters (integrated transgenes or antibodies) were used to mark certain tissues,  subcellular structures or life stages, etc. as a reference point to assay gene function or location.||wchen@its.caltech.edu, vanauken@its.caltech.edu
+|||||colspan="6"|INTERACTIONS:
 |-
-|||Regulation of gene expression patterns:
+|||||'''Genetic interactions''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=geneinteractions (flagged-done)]||''Gene interactions'' ||geneint||''Check if your paper reports the analysis of more than one gene at a time, e.g., double, triple, etc. mutants, including experiments where RNAi was concurrent with other RNAi-treatments or mutations.''||remove '''emsch@its.caletch.edu''' ||
 |-
-|in progress||||'''Gene expression altered by genetic background or other treatment'''  [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=generegulation (flagged-done)]||''Gene regulation on expression level'' ; generegulation ||Please indicate if your paper reports changes or lack of changes in gene expression levels or patterns due to genetic background, exposure to chemicals or temperature or any other experimental treatment.||xdwang@its.caltech.edu
+|||materials and methods (tools); results||'''Functional complementation''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=functionalcomplementation (flagged)]||''Functional Complementation'' ||funccomp||Check if your paper reports functional redundancy between separate genes, e.g. the rescue of ''gen-A'' by overexpression of ''gen-B'' or any other extragenic sequence.|| ||
 |-
-|||||'''Regulatory sequence features'''  [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=sequencefeatures (flagged)]||''Sequence features'' ; sequencefeatures ||Please indicate if your paper reports any gene expression regulatory elements such as DNA/RNA elements required for gene expression,  promoters, introns, UTR's, DNA binding sites, etc.||xdwang@its.caltech.edu, worm-bug@sanger.ac.uk, stlouis@wormbase.org
+|||||'''Gene product interactions''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=geneproduct (flagged-done)]||''Gene product interaction'' ||geneprod||Check if your paper reports data on protein-protein, RNA-protein, DNA-protein or Y2H interactions, etc.|| remove '''emsch@its.caletch.edu''' ||
 |-
-|||||'''Position frequency matrix (PFM)''' or '''Postition weight matrix (PWM)'''||'''new field''' = matrices||Please indicate if your paper reports PFMs or PWMs that are typically used to define regulatory sites in genomic DNA (e.g., bound by transcription factors) or mRNA (e.g., bound by translational factors or miRNA). PFMs define simple nucleotide frequencies, while PWMs are scaled logarithmically against a background frequency.||xdwang@its.caltech.edu, emsch@its.caltech.edu
+|||||colspan="6"|REGULATION OF GENE EXPRESSION:
 |-
-|||||'''Mosaic analysis''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=mosaic (flagged-done)]||''Mosaic analysis'' ; mosaic ||Please indicate if your paper reports cell specific gene function based on mosaic analysis, e.g. extra-chromosomal transgene loss in a particular cell lineage leads to loss of mutant rescue, etc. ||raymond@its.caltech.edu
+|some SVM (not great)||||'''New expression pattern for a gene''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=expression (flagged-done)]||''expression pattern data''|| otherexpr ||Check if your paper reports new temporal or spatial (e.g., tissue, subcellular, etc.) data on the pattern of expression of any gene in a wild-type background. You can include:  reporter gene analysis, antibody staining, ''In situ'' hybridization, RT-PCR, Western or Northern blot data.||wchen@its.caltech.edu, vanauken@its.caltech.edu||
 |-
-||||| '''Tissue or cell site of action''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=site (flagged-done)]||''Site of action'' ; site ||Please indicate if your paper reports anatomy(tissue/cell)-specific expression function for a gene.||raymond@its.caltech.edu
+|some SVM (not great)||||'''Alterations in gene expression by genetic or other treatment''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=generegulation (flagged-done)]||''Gene regulation on expression level'' || genereg ||Check if your paper reports changes or lack of changes in gene expression levels or patterns due to genetic, chemical, temperature, or any other experimental treatment.||xdwang@its.caltech.edu ||
 |-
-|||||'''Developmental time of action'''||'''new field''' = timeofaction||Please indicate if your paper reports a temporal requirement for gene function.||raymond@its.caltech.edu
+|||||'''Regulatory sequence features'''  [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=sequencefeatures (flagged)]||''Sequence features'' ||seqfeat ||Check if your paper reports any gene expression regulatory elements, e.g., DNA/RNA elements required for gene expression,  promoters, introns, UTR's, DNA binding sites, etc.||xdwang@its.caltech.edu, worm-bug@sanger.ac.uk, stlouis@wormbase.org ||
 |-
-|||||'''Microarray'''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=microarray (flagged-done)]||''Microarray'' ; microarray ||Please indicate if your paper reports any microarray data.||wchen@its.caltech.edu
+|||||'''Position frequency matrix (PFM)''' or '''Position weight matrix (PWM)'''||'''new field''' || matrices||Check if your paper reports PFMs or PWMs, which are typically used to define regulatory sites in genomic DNA (e.g., bound by transcription factors) or mRNA (e.g., bound by translational factors or miRNA). PFMs define simple nucleotide frequencies, while PWMs are scaled logarithmically against a background frequency.||xdwang@its.caltech.edu, remove- '''emsch@its.caletch.edu''' ||
 |-
-|||PROTEIN FUNCTION AND STRUCTURE:
+|||||'''Microarray'''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=microarray (flagged-done)]||''Microarray''|| microarray ||Check if your paper reports any microarray data.||wchen@its.caltech.edu ||
 |-
-|||||'''Protein Analysis ''in vitro'''''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=invitro (flagged)]||in vitro ''Protein analysis''; invitro ||Please indicate if your paper reports any ''in vitro'' protein analysis including such things as kinase assays, agonist pharmacological studies, ''in vitro reconstitution studies, etc.||
+|||||colspan="6"|PROTEIN FUNCTION AND STRUCTURE:
 |-
-|||||'''Domain Analysis'''||'''new field''' = domainanalysis||Please indicate if your paper reports on a function of a particular domain within a protein.||
+|Kimberly said to remove this ||materials and methods; results||'''Protein analysis ''in vitro'''''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=invitro (flagged)]||in vitro ''Protein analysis''|| invitro ||Check if your paper reports any ''in vitro'' protein analysis such as kinase assays, agonist pharmacological studies, ''in vitro'' reconstitution studies, etc.|| ||
 |-
-|||||'''Covalent Modification''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=covalent (flagged)]||''Covalent modification'' ; covalent|| Please indicate if your paper reports on post-translational modifications as assayed by mutagenesis or ''in vitro'' analysis||
+|||materials and methods; results||'''Domain analysis'''||'''new field''' || domanal (populated with information previously in "structureinformation")||Check if your paper reports on a function of a particular domain within a protein.||||
 |-
-|||||'''Structural Information '''Structural information''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=structureinformation (flagged)]: ||NMR structure, functional domain info for a protein ||''"removal of the first 50aa causes mislocalization of the protein"''; ''"fig.1, fig.8"''; ''"yes, in paper and supplemental materials"''; ''"FIGURE 5. The let-7 sequence is required for formation of the M1 and M2 complexes."''; ''"functional domains of gld-2, fig 3"''; ''"Fig. 3. Comparison of RDE-4 binding properties to variants lacking, or with mutations in, dsRBM1."'' ||
+|||materials and methods; results||'''Covalent modification''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=covalent (flagged)]||''Covalent modification'' || covalent|| Check if your paper reports on post-translational modifications as assayed by mutagenesis or ''in vitro'' analysis||||
 |-
-||| Functional Complementation '''Functional Complementation''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=functionalcomplementation (flagged)]: ||Functional redundancy, rescue by overexpression of extragenic sequence ||''"exc-2 is rescued by exc-9 overexpression"''; ''"...meg-2 functions redundantly with meg-1. Each transgene can rescue the sterility of meg-1(vr10) or meg-1(vr11)... The partial rescue of meg-1 mutants by GFPTMEG-2 suggests that extra copies of MEG-2 can compensate for the absence of MEG-1, implying that the overall level of MEG-1 and MEG-2 is important for proper germline development."''; ''"In transformation experiments, we identified a cosmid, C26G6, which could rescue the egl-32 phenotype. Subclones of this cosmid containing the predicted open reading frame (ORF) T08G11.2 can also rescue egl-32 (Figures 3a &amp; b). Several lines of evidence, however, suggest that egl-32 does not encode T08G11.2, but rather that they are interacting loci"''||
+|||materials and methods; results||'''Structural information'''[http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=structureinformation (flagged)]||''Structure information''|| structinfo||Check if your paper reports NMR or X-ray crystallographic information.|||| besides structure info (e.g. x-ray crystallography data) Andrei also includes structure-function data (e.g. mutation at Ser-321 compromises folding, binding, etc.)
 |-
+|||||'''Mass spectrometry''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=massspec (flagged-done)]||''Mass Spec''|| massspec||Check if your paper reports data from any mass spec analysis; keywords: mass spectrometry, peptide, (and any one of the following:) MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix.||gw3@ebi.ac.uk, worm-bug@sanger.ac.uk||From Gary "...only interested in papers that report the peptide sequences that the mass-spec fragments match. These peptides are usually created by one of the programs: MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix. So, the Description field should be:
+Keywords: mass spectrometry, peptide, (and any one of the following:) MASCOT, SEQUEST, X!Tandem, OMSSA, MassMatrix
-||| Covalent Modification '''Covalent modification''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=covalent (flagged)]: ||phosphorylation site is studies via mutagenesis and in vitro assay ||''"Analysis of cDNA sequences derived from the eri-7 pre-mRNA stabilized in rnp-5 RNAi-treated animals revealed adenosine to guanosine transitions at four positions located within the direct repeat (Fig. 2d). These transitions are indicative of adenosine to inosine editing of the eri-7 59-UTR by an adenosine deaminase (ADAR)24"''
 |-
-||| Non-N2_phenotype : ||Phenotypes of strains/non-C. elegans||||
+|||||colspan="6"|'''REAGENTS''':
+|-
+|'''DONE'''||||'''''C. elegans'' antibodies''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=antibody (flagged-done)]||''Extract Antibody''|| antibody ||Check if your paper reports the use of new or known antibodies created by your lab or someone else's lab; do not check this box if antibodies were commercially bought.||wchen@its.caltech.edu ||
+|-
+|'''DONE'''||||'''Integrated transgenes''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=transgene (flagged-done)] ||''Transgene''||transgene||Check if integrated transgenes were used in this paper. If the transgene does not have a canonical name, please list it in the "Add Information text area" ||wchen@its.caltech.edu ||
+|-
+|||||'''Transgenes used as tissue markers'''||''Marker''|| marker||Check if reporters (integrated transgenes) were used to mark certain tissues,  subcellular structures, or life stages, etc. as a reference point to assay gene function or location.||wchen@its.caltech.edu, vanauken@its.caltech.edu ||
+|-
+|||||colspan="6"|GENOME SEQUENCE DATA:
+|-
+|||||'''Gene structure correction''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=structurecorrectionsanger (flagged)]||''Sanger Gene Structure Correction'' and ''St. Louis Gene Structure Correction''|| structcorr (this use to be two different fields)||Check if your paper reports a gene structure that is different from the one in WormBase, e.g.,  different splice-site, SL1 instead of SL2, etc.||worm-bug@sanger.ac.uk, wormticket@watson.wustl.edu||
+the authors may or may not state explicitly that let's say there is a
+novel exon. if i see a gene studied in some detail (e.g. new gene was
+cloned or gene structure is drawn in fig.), than i check amino acid
+length for the protein with the data in WB, and i will eyeball the
+diagrams of gene structures to see if there are obvious diffs. these
+are quick checks but they catch an occasional gene structure change
+not listed in the text.
+|-
+|||||'''Sequencing mutant alleles''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=sequencechange (flagged)]||''Sequence change''||seqchange ||Check if your paper reports new sequence data for any mutation.||genenames@wormbase.org||
 |-
-||| Sequence Change '''Sequencing mutant alleles''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=sequencechange (flagged)]: ||Mutation was sequenced ||''"the hcf- 1(pk924) mutant has a large deletion that should result in a frame shift leading to an early stop codon, and likely represents a null mutant (Figure S1) [35]."''; ''"table 2: unnamed mutations"''; ''"FIGURE 5. Predicted structure of the glo-3 gene and encoded protein. (A) The structure of the glo-3 gene and the location and phenotypic class of mutations are shown"''; ''"lin-15 mutation p.834"'' ||genenames@wormbase.org
+|||||'''New SNPs''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=newsnp (flagged)]||''Extract New SNP''||newsnp||Check if your paper reports a SNP that does not already exist in WormBase.||dblasiar@watson.wustl.edu, tbieri@watson.wustl.edu||
 |-
-||| Gene Interaction and Epistasis '''Genetic interactions''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=geneinteractions (flagged-done)]: ||analysis of more than one gene at a time, e.g. double, triple, etc. mutants, RNAi concurrent with other RNAi-treated worms or mutants||''"e.g. daf-16(mu86) suppresses daf-2(e1370), daf-16(RNAi) suppresses daf-2(RNAi)"''; ''"hcf-1, daf-16'';''daf-18, smg-1"''; ''"eri-6, eri-7"''; ''"gene interactions large-scale, table"''; ''"Epistasis analysis in figure 2 and table 2"'' ||emsch@its.caltech.edu
+|||||colspan="5"|CELL DATA:
 |-
-||| Gene Product Interaction '''Gene product interactions''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=geneproduct (flagged-done)]: ||protein-protein, RNA-protein, DNA-protein interactions, Y2H, etc., ||''"Table S4. PDZ domain specificity prediction"''; ''"Figure 5. Loss of hcf-1 Promotes the DAF-16 transcriptional Regulation of Several Target Genes...Figure 6. HCF-1 Forms a Protein Complex with DAF-16 in C. elegans..."''; ''"Interestingly, the eri-6/7 transsplicing reporter is more highly and broadly expressed when RNAi is attenuated by inactivation of the Argonaute gene rde-1 (Supplementary Fig. 12), suggesting that the eri-6/7 is a target of RNAi..."''; ''"Fig. 1. Identification of genes that regulate clec-85::gfp expression"'' || emsch@its.caltech.edu
+|||||'''Ablation data''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=ablationdata (flagged-done)]||''Ablation data''||ablationdata ||Check if your paper reports data from an assay involving any cell or anatomical unit being ablated by laser or by other means (e.g., by expressing a cell-toxic protein).||raymond@its.caltech.edu ||
 |-
-||| Sanger Gene Structure Correction '''Gene structure correction''' - need to make sure Sanger is responsible for the clone [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=structurecorrectionsanger (flagged)]: ||Gene Structure Correction (Gene Structure is different from the one in Wormbase: e.g. different splice-site, SL1 instead of SL2, etc.)||''"...JA:F59F5.2 targets two predicted genes, F59F5.2 and F59F5.8. Two previously isolated cDNAs, yk1328a05 and yk571h2, suggested that F59F5.2 and F59F5.8 are a single gene that is alternatively spliced to produce two transcripts. We independently isolated F59F5.2/.8 cDNAs from both adult and embryonic stages, supporting the conclusion that F59F5.2 and F59F5.8 are a single gene (see MATERIALS AND METHODS). We refer to the long F59F5.2/.8 transcript as glo-3 and the F59F5.2 transcript as glo-3 short (Figure 5A)."'' ||worm-bug@sanger.ac.uk
+|||||'''Cell function''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=cellfunction (flagged-done)]||''Cell function''||cellfunc||Check if your paper reports a function for any anatomical part (e.g., cell, tissue, etc.), which has not been indicated elsewhere on this form.||raymond@its.caltech.edu ||
 |-
-||| St. Louis Gene Structure Correction '''Gene structure correction''' - need to make sure StLouis is responsible for the clone [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=structurecorrectionstlouis (flagged)]: ||Gene Structure Correction (Gene Structure is different from the one in Wormbase: e.g. different splice-site, SL1 instead of SL2, etc.)||''"C41D11.1 and C41D11.7 fig.1"''; ''"We confirmed two of three forms by isolation of cDNAs (gcy-28.a and gcy-28.c, corresponding to T01A4.1a and T01A4.1c, respectively) and identified a fourth splice form, T01A4.1d (gcy-28.d), which fuses the upstream predicted gene T01A4.2 to T01A4.1 (Figure 4A)."''; ''"page 3: By contrast, 235 of the indels occurred in regions with no perfectly aligning Solexa read, suggesting a possible error in the C. elegans reference genome,"''||wormticket@watson.wustl.edu
+|||||colspan="5" |IN SILICO DATA:
 |-
+||||||'''Phylogenetic data'''||'''new field'''||phylogenetic||Check if your paper reports any phylogenetic analysis.||||
-||| Mass Spec '''Mass spectrometry''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=massspec (flagged-done)]: ||key words: LCMS, COSY, mass spec, HRMS||||gw3@sanger.ac.uk, worm-bug@sanger.ac.uk
 |-
-||| Cell/Anatomy Function '''Cell function''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=cellfunction (flagged-done)]: ||Function of any anatomical part (e.g. cell) is mentioned that has not been flagged already for mosaic analysis, site of action, or ablation data||''"Figure 3 and Supp table 2 have information on predicted navigation circuit."'' ||raymond@its.caltech.edu
+||||||'''Other bioinformatics analysis'''||'''new field'''||othersilico||Check if your paper reports any bioinformatic data not indicated anywhere else on this form.||||
 |-
-||| Ablation Data '''Ablation data''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=ablationdata (flagged-done)]: ||cell or anatomical unit was ablated using a laser or by other means (e.g. by expressing a cell-toxic protein)||''"Killing AWCON in wild-type animals abolished the net migration toward butanone (Figure 3A; Wes and Bargmann, 2001"''||raymond@its.caltech.edu
+|||||colspan="5"|OTHER:
 |-
-||| Extract New SNP '''New SNPs''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=newsnp (flagged)]: ||Reagent: new SNP not already in WB||''"page 3: By contrast, 235 of the indels occurred in regions with no perfectly aligning Solexa read, suggesting a possible error in the C. elegans reference genome,"''||dblasiar@watson.wustl.edu, tbieri@watson.wustl.edu
+|||||'''Supplemental materials''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=supplemental (flagged-done)]||''Supplemental material''||supplemental||Check if your paper has supplemental material.||qwang@its.caltech.edu ||
 |-
-|retired? || Extract SNP Verified by St. Louis [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=stlouissnp (flagged)]: ||Authors report reference genome is incorrect||''"fig.2: two SNPs mentioned"''; ''any SNP mentioned''; ''"For nekl-1, cDNA clones indicated that the predicted gene annotation was incorrect."'' ||dblasiar@watson.wustl.edu, tbieri@watson.wustl.edu
+|||||'''NONE of the aforementioned data types are in this research article'''  [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=comment (flagged)]||'''Comment'''||nocuratable||Check if none of the above pertains to your paper. Feel free to list the data type most pertinent to your research paper in the "Add information" text area.||||
 |-
-||| Supplemental Material '''Supplemental materials''' [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fc&field=supplemental (flagged-done)]: ||Flag if supplemental material was not already downloaded. |||''yes''||qwang@its.caltech.edu
+|||||'''Any feedback? Please feel free to give us feedback for this form or for any other topic pertinent to how we can better extract data from your paper.''' ||'''new field'''||comment||Comments from all authors and curators are accessible through the "Comment" button at the bottom of the page.||kyook@caltech.edu, vanauken@caltech.edu||
 |-
+|}
+--[[User:Kyook|kjy]] 17:56, 29 July 2010 (UTC)
-||| Comment [http://tazendra.caltech.edu/~postgres/cgi-bin/curation_status.cgi?action=fnc&field=comment (flagged)]: ||''e.g. no curatable'';''review'';''the paper is used for functional annotations''||||''stays in Postgres''
+[[Category:Curation]]
-|}

Difference between revisions of "Texpresso/Author/Curator interim form"

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