Summary of Study ST000353

This data is available at the NIH Common Fund's National Metabolomics Data Repository (NMDR) website, the Metabolomics Workbench, https://www.metabolomicsworkbench.org, where it has been assigned Project ID PR000282. The data can be accessed directly via it's Project DOI: 10.21228/M8G308 This work is supported by NIH grant, U2C- DK119886.

See: https://www.metabolomicsworkbench.org/about/howtocite.php

Study ID	ST000353
Study Title	The Development of Metabolomic Markers in African Bermudagrass (C. transvaalensis) for Sting Nematode (Belonolaimus longicaudatus) Response
Study Type	Disease response in terms of nematode reproduction and root weight
Study Summary	The objective of the proposed pilot study is to identify metabolites up- and down-regulated in African bermudagrass that are tolerant and sensitive to the sting nematode and develop metabolomic markers for the highest expressed metabolites associated with tolerance. Future work will include additional accessions and species of bermudagrass, and testing under field conditions. Bermudagrass accessions identified as tolerant or sensitive by Pang et al. (2011) will be assessed under controlled greenhouse conditions to identify metabolites linked to sting nematode tolerance. Nematode response will be quantified through determination of root length and weight and the number of nematodes present 136 days after inoculation. Higher root length and weight indicate tolerance or resistance. Higher nematode counts indicate greater reproduction (i.e. a susceptible plant), while lower counts indicate that the accession may have some resistance. Metabolites from root tissue of these accessions will be compared to identify those associated with tolerance/resistance, and those that are associated with nematode infestation by comparing inoculated plants to uninoculated controls. Metabolomic markers will then be developed for the metabolites associated with tolerance/resistance. These markers will be used to guide future screening of bermudagrass accessions for breeding nematode-tolerant or -resistant varieties.
Institute	University of Florida
Department	SECIM
Laboratory	Turfgrass Breeding
Last Name	Benda
First Name	Nicole
Address	2005 SW 23rd St
Email	nbenda@ufl.edu
Phone	352-792-4561
Submit Date	2015-11-13
Num Groups	3
Total Subjects	42
Raw Data Available	Yes
Raw Data File Type(s)	mzML
Analysis Type Detail	LC-MS
Release Date	2017-07-10
Release Version	1

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Project:

Project ID:	PR000282
Project DOI:	doi: 10.21228/M8G308
Project Title:	The Development of Metabolomic Markers in Bermudagrass (Cynodon spp.) for Sting Nematode (Belonolaimus longicaudatus) Response
Project Summary:	The majority of golf courses in Florida experience damage from plant-parasitic nematodes and more than 80% of golf courses in Florida are at risk for nematode-related damage (Crow, 2005). With limited availability of nematicides and lack of tolerant cultivars, turf managers need new genetically resistant cultivars. Use of resistant or tolerant grasses is the most efficient, environmentally friendly and, in the long run, least costly component of IPM. Current screening of new genotypes for nematode resistance is labor- and time-intensive, with three months required soley for nematode development on test plants. We intend to develop metabolomic markers or a signature pattern associated with nematode resistance or tolerance. Screening plants for these markers or a signature pattern of would greatly speed up the screening process and development of resistant cultivars.
Institute:	University of Florida
Department:	Agronomy
Laboratory:	Turfgrass Breeding
Last Name:	Kenworthy
First Name:	Kevin
Address:	2005 SW 23rd Street, Gainesville FL 32611
Email:	nbenda@ufl.edu
Phone:	352-792-4561

Subject:

Subject ID:	SU000373
Subject Type:	Plant
Subject Species:	Cynodon transvaalensis
Taxonomy ID:	75728
Genotype Strain:	AB03, AB33, and AB39
Age Or Age Range:	4 month old plant clones
Subject Comments:	(African Bermudagrass,C. transvaalensis)
Species Group:	Plant

Factors:

Subject type: Plant; Subject species: Cynodon transvaalensis (Factor headings shown in green)

mb_sample_id	local_sample_id	Plant genotype	Nematode inoculation
SA015451	AB03_I_13	AB03	inoc
SA015452	AB03_I_1	AB03	inoc
SA015453	AB03_I_10	AB03	inoc
SA015454	AB03_I_7	AB03	inoc
SA015455	AB03_I_2	AB03	inoc
SA015456	AB03_I_4	AB03	inoc
SA015457	AB03_I_5	AB03	inoc
SA015458	AB03_U_14	AB03	uninoc
SA015459	AB03_U_8	AB03	uninoc
SA015460	AB03_U_11	AB03	uninoc
SA015461	AB03_U_7	AB03	uninoc
SA015462	AB03_U_6	AB03	uninoc
SA015463	AB03_U_4	AB03	uninoc
SA015464	AB03_U_3	AB03	uninoc
SA015465	AB33_I_10	AB33	inoc
SA015466	AB33_I_11	AB33	inoc
SA015467	AB33_I_8	AB33	inoc
SA015468	AB33_I_5	AB33	inoc
SA015469	AB33_I_3	AB33	inoc
SA015470	AB33_I_1	AB33	inoc
SA015471	AB33_I_2	AB33	inoc
SA015472	AB33_U_11	AB33	uninoc
SA015473	AB33_U_9	AB33	uninoc
SA015474	AB33_U_13	AB33	uninoc
SA015475	AB33_U_2	AB33	uninoc
SA015476	AB33_U_8	AB33	uninoc
SA015477	AB33_U_4	AB33	uninoc
SA015478	AB33_U_7	AB33	uninoc
SA015479	AB39_I_11	AB39	inoc
SA015480	AB39_I_9	AB39	inoc
SA015481	AB39_I_12	AB39	inoc
SA015482	AB39_I_8	AB39	inoc
SA015483	AB39_I_3	AB39	inoc
SA015484	AB39_I_1	AB39	inoc
SA015485	AB39_I_4	AB39	inoc
SA015486	AB39_U_9	AB39	uninoc
SA015487	AB39_U_10	AB39	uninoc
SA015488	AB39_U_7	AB39	uninoc
SA015489	AB39_U_5	AB39	uninoc
SA015490	AB39_U_2	AB39	uninoc
SA015491	AB39_U_3	AB39	uninoc
SA015492	AB39_U_6	AB39	uninoc

Showing results 1 to 42 of 42

Showing results 1 to 42 of 42

Collection:

Collection ID:	CO000367
Collection Summary:	Rinsed roots were cut off the plant, placed into paper envelopes, and immediately placed into liquid nitrogen. Roots were stored at -80°C until freeze-drying. Freeze-dried roots were held at room temperature in ziploc bags with silica gel packets. They were then frozen in liquid nitrogen and ground to a powder in a tissue homogenizer with ball bearings (Geno/Grinder 2010), and then stored in 2 ml snap-cap plastic tubes at room temperature.
Sample Type:	plant root tissue
Collection Method:	whole plant destruction
Collection Location:	greenhouse
Collection Frequency:	once
Collection Duration:	1-2 minutes to cut off and rinse the roots prior to placement into liquid nitrogen
Collection Time:	136 days after inoculation
Volumeoramount Collected:	0.2-0.5 grams of root tissue, dry weight
Storage Conditions:	1)-80C until freeze-drying. 2) Held at room temperature in ziploc bags with silica packets. 3) Frozen in liquid nitrogen and ground using a Geno/Grinder 2010. 4) Transferred to 2 mL tubes and held at room temperature.
Collection Vials:	Paper coin envelopes
Storage Vials:	2 ml snap-cap plastic tubes
Collection Tube Temp:	liquid nitrogen (-196°C)
Additives:	none

Treatment:

Treatment ID:	TR000387
Treatment Summary:	Plants clones propagated by stolons were allowed to establish for 30 days in 4 cm diameter conetainers filled with sand. Fifty sting nematodes (mixed age and gender) were added to each conetainer and allowed to grow and reproduce for 90 days. Nematodes were then rinsed off of roots for quantification, and plant roots were frozen in liquid nitrogen and stored at -80C until they were freeze-dried.Freeze-dried roots were ground to a powder and then submitted for global metabolomic analysis.
Treatment:	Biotic
Treatment Compound:	Sting nematode, Belonolaimus longicaudatus
Plant Growth Support:	sand in conetainers- 4 cm wide, 30 cm deep
Plant Growth Location:	temperature controlled greenhouse
Plant Plot Design:	complete randomized design
Plant Light Period:	Natural lighting, ca. 11:13 Light:Dark
Plant Humidity:	ca.50%RH
Plant Temp:	25°C
Plant Watering Regime:	Twice daily for 5 min
Plant Nutritional Regime:	Weekly liquid fertilizer of 24-8-16 (N-P-K)
Plant Estab Date:	2015-09-24
Plant Harvest Date:	2016-04-02
Plant Growth Stage:	non-reproductive
Plant Metab Quench Method:	liquid nitrogen, followed by storage at -80°C
Plant Harvest Method:	rinsed roots were cut off the plant and placed into paper envelopes
Plant Storage:	1)-80C until freeze-drying. 2) Held at room temperature in ziploc bags with silica packets. 3) Frozen in liquid nitrogen and ground using a Geno/Grinder 2010. 4) Transferred to 2 mL tubes and held at room temperature.

Sample Preparation:

Sampleprep ID:	SP000380
Sampleprep Summary:	none
Sampleprep Protocol Filename:	Maize_Tissue_sample_prep.pdf

Combined analysis:

Analysis ID	AN000575	AN000576
Analysis type	MS	MS
Chromatography type	Reversed phase	Reversed phase
Chromatography system	Thermo Scientific-Dionex Ultimate 3000	Thermo Scientific-Dionex Ultimate 3000
Column	ACE Excel 2 C18-PFP (100 x 2.1mm, 2um)	ACE Excel 2 C18-PFP (100 x 2.1mm, 2um)
MS Type	ESI	ESI
MS instrument type	Orbitrap	Orbitrap
MS instrument name	Thermo Q Exactive Orbitrap	Thermo Q Exactive Orbitrap
Ion Mode	POSITIVE	NEGATIVE
Units	peak area	peak area

Chromatography:

Chromatography ID:	CH000411
Chromatography Summary:	See document
Methods Filename:	Metabolomics_LCMSProtocol.pdf Appendix_A_-_Internal_Standard_Prep_GLCMS.pdf
Instrument Name:	Thermo Scientific-Dionex Ultimate 3000
Column Name:	ACE Excel 2 C18-PFP (100 x 2.1mm, 2um)
Flow Rate:	0.350mL/min-0.600mL/min
Internal Standard:	Appendix A - Internal Standard Prep GLCMS.pdf
Solvent A:	100% water; 0.1% formic acid
Solvent B:	100% acetonitrile
Chromatography Type:	Reversed phase

MS:

MS ID:	MS000511
Analysis ID:	AN000575
Instrument Name:	Thermo Q Exactive Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	HESI
Ion Mode:	POSITIVE
Analysis Protocol File:	Metabolomics_LCMSProtocol.pdf

MS ID:	MS000512
Analysis ID:	AN000576
Instrument Name:	Thermo Q Exactive Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	HESI
Ion Mode:	NEGATIVE
Analysis Protocol File:	Metabolomics_LCMSProtocol.pdf