Summary of Study ST003279

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 PR002032. The data can be accessed directly via it's Project DOI: 10.21228/M8ZC0C This work is supported by NIH grant, U2C- DK119886.

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

This study contains a large results data set and is not available in the mwTab file. It is only available for download via FTP as data file(s) here.

Study ID	ST003279
Study Title	Metabolomic analysis of Axon Regeneration in Xenopus laevis Tectum
Study Summary	We profile the metabolite changes in the tectum of a transgenic line of 1 year old Xenopus laevis Tg(islet2b:gfp) frogs that either had a monocular surgery of either a left optic crush injury (crush) or sham surgery (sham). The matching controls of uninjured right optic nerves were also collected (control). Tg(islet2b:gfp) frogs were allowed to recover for 12 and 27 days post optic nerve crush. Following euthanasia, the tissues were collected for metabolomic analysis. Samples were pooled for each category (crush, sham, and control) at n =3 to obtain sufficient metabolite concentrations for analysis. Metabolites were extracted using a Precellys Homogenizer and a serial extraction method: (1) 1:1 Methanol/Water and (2) 8:1:1 Acetonitrile/Methanol/Acetone. Metabolites were analyzed by untargeted liquid chromatography-mass spectrometry (LC MS-MS) profiling using a Q-Exactive Orbitrap instrument coupled with Vanquish Horizon Binary UHPLC LC-MS system. Metabolites were identified and quantified using Compound Discoverer 3.3 and isotopic internal metabolites standards.
Institute	University of Miami
Department	McKnight - Ophthalmology
Laboratory	Bhattacharya Lab
Last Name	Bhattacharya
First Name	Sanjoy
Address	1638 NW 10th Avenue, Room 706-A, Miami, FL 33136
Email	sbhattacharya@med.miami.edu
Phone	3054824103
Submit Date	2024-06-05
Raw Data Available	Yes
Raw Data File Type(s)	raw(Thermo)
Analysis Type Detail	LC-MS
Release Date	2024-07-15
Release Version	1

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Project:

Project ID:	PR002032
Project DOI:	doi: 10.21228/M8ZC0C
Project Title:	Metabolomic Analysis of Axon Regeneration in Xenopus laevis
Project Summary:	CNS injuries of the anuran amphibian, Xenopus laevis, are uniquely befitted for studying the molecular compositions of neuronal regeneration of retinal ganglion cells (RGC) due to a functional recovery of optic axons disparate to adult mammalian analogues. RGCs and their optic nerve axons undergo irreversible neurodegeneration in glaucoma and associated optic neuropathies, resulting in blindness in mammals. Conversely, Xenopus demonstrates RGC lifetime-spanning regenerative capabilities after optic nerve crush, inciting opportunities to compare de novo regeneration and develop efficient pharmaceutical approaches for vision restoration. Studies revealing metabolome alterations during optic nerve regeneration are sparse and could serve as a solid foundation for these underlying molecular changes. We profile the metabolite changes in the optic tissues of a transgenic line of 1 year old Xenopus laevis Tg(islet2b:gfp) frogs that either had a monocular surgery of either a left optic crush injury (crush) or sham surgery (sham). The matching controls of uninjured right optic nerves were also collected (control). Tg(islet2b:gfp) frogs were allowed to recover for 12 and 27 days post optic nerve crush. Following euthanasia, the tissues were collected for metabolomic analysis. Samples were pooled for each category (crush, sham, and control) at n =3 to obtain sufficient metabolite concentrations for analysis. Metabolites were extracted using a Precellys Homogenizer and a serial extraction method: (1) 1:1 Methanol/Water and (2) 8:1:1 Acetonitrile/Methanol/Acetone. Metabolites were analyzed by untargeted liquid chromatography-mass spectrometry (LC MS-MS) profiling using a Q-Exactive Orbitrap instrument coupled with Vanquish Horizon Binary UHPLC LC-MS system. Metabolites were identified and quantified using Compound Discoverer 3.3 and isotopic internal metabolites standards.
Institute:	University of Miami
Department:	McKnight - Ophthalmology
Laboratory:	Bhattacharya Lab
Last Name:	Bhattacharya
First Name:	Sanjoy
Address:	1638 NW 10th Avenue, Room 706-A, Miami, FL 33136
Email:	sbhattacharya@med.miami.edu
Phone:	3054824103

Subject:

Subject ID:	SU003399
Subject Type:	Amphibian
Subject Species:	Xenopus laevis
Taxonomy ID:	8355

Factors:

Subject type: Amphibian; Subject species: Xenopus laevis (Factor headings shown in green)

mb_sample_id	local_sample_id	Sample source	Treatment
SA354885	Blank_NEG3	NA	Extraction Blank
SA354886	Blank_POS2	NA	Extraction Blank
SA354887	Blank_POS1	NA	Extraction Blank
SA354888	Blank_NEG2	NA	Extraction Blank
SA354889	Blank_POS3	NA	Extraction Blank
SA354890	Blank_NEG1	NA	Extraction Blank
SA354891	CTL_27dpi_Tect1_NEG2	Tectum	Control
SA354892	CTL_27dpi_Tect3_NEG3	Tectum	Control
SA354893	CTL_27dpi_Tect3_NEG2	Tectum	Control
SA354894	CTL_27dpi_Tect3_NEG1	Tectum	Control
SA354895	CTL_27dpi_Tect3_POS3	Tectum	Control
SA354896	CTL_27dpi_Tect3_POS2	Tectum	Control
SA354897	CTL_27dpi_Tect3_POS1	Tectum	Control
SA354898	CTL_27dpi_Tect2_NEG3	Tectum	Control
SA354899	CTL_27dpi_Tect2_NEG2	Tectum	Control
SA354900	CTL_27dpi_Tect2_NEG1	Tectum	Control
SA354901	CTL_27dpi_Tect2_POS3	Tectum	Control
SA354902	CTL_27dpi_Tect2_POS1	Tectum	Control
SA354903	CTL_27dpi_Tect1_NEG3	Tectum	Control
SA354904	CTL_27dpi_Tect2_POS2	Tectum	Control
SA354905	CTL_27dpi_Tect1_NEG1	Tectum	Control
SA354906	CTL_12dpi_Tect2_POS1	Tectum	Control
SA354907	CTL_12dpi_Tect1_POS1	Tectum	Control
SA354908	CTL_12dpi_Tect1_POS2	Tectum	Control
SA354909	CTL_12dpi_Tect1_POS3	Tectum	Control
SA354910	CTL_27dpi_Tect1_POS3	Tectum	Control
SA354911	CTL_12dpi_Tect1_NEG2	Tectum	Control
SA354912	CTL_12dpi_Tect1_NEG3	Tectum	Control
SA354913	CTL_12dpi_Tect1_NEG1	Tectum	Control
SA354914	CTL_12dpi_Tect2_POS2	Tectum	Control
SA354915	CTL_12dpi_Tect2_NEG1	Tectum	Control
SA354916	CTL_12dpi_Tect2_NEG2	Tectum	Control
SA354917	CTL_12dpi_Tect2_NEG3	Tectum	Control
SA354918	CTL_27dpi_Tect1_POS2	Tectum	Control
SA354919	CTL_27dpi_Tect1_POS1	Tectum	Control
SA354920	CTL_12dpi_Tect2_POS3	Tectum	Control
SA354921	CX_27dpi_Tect2_POS1	Tectum	Crush
SA354922	CX_27dpi_Tect1_NEG1	Tectum	Crush
SA354923	CX_27dpi_Tect1_NEG3	Tectum	Crush
SA354924	CX_27dpi_Tect2_NEG1	Tectum	Crush
SA354925	CX_27dpi_Tect2_POS2	Tectum	Crush
SA354926	CX_27dpi_Tect2_POS3	Tectum	Crush
SA354927	CX_27dpi_Tect2_NEG2	Tectum	Crush
SA354928	CX_27dpi_Tect2_NEG3	Tectum	Crush
SA354929	CX_27dpi_Tect1_POS1	Tectum	Crush
SA354930	CX_27dpi_Tect1_POS2	Tectum	Crush
SA354931	CX_27dpi_Tect1_NEG2	Tectum	Crush
SA354932	CX_12dpi_Tect2_NEG3	Tectum	Crush
SA354933	CX_12dpi_Tect1_NEG1	Tectum	Crush
SA354934	CX_12dpi_Tect2_NEG2	Tectum	Crush
SA354935	CX_12dpi_Tect1_POS1	Tectum	Crush
SA354936	CX_12dpi_Tect1_POS2	Tectum	Crush
SA354937	CX_12dpi_Tect1_POS3	Tectum	Crush
SA354938	CX_27dpi_Tect1_POS3	Tectum	Crush
SA354939	CX_12dpi_Tect1_NEG2	Tectum	Crush
SA354940	CX_12dpi_Tect2_POS1	Tectum	Crush
SA354941	CX_12dpi_Tect2_POS2	Tectum	Crush
SA354942	CX_12dpi_Tect2_POS3	Tectum	Crush
SA354943	CX_12dpi_Tect1_NEG3	Tectum	Crush
SA354944	CX_12dpi_Tect2_NEG1	Tectum	Crush
SA354945	Pooled_QC2_MS1_Tect_POS1	Tectum	QC
SA354946	Pooled_QC1_MS2_Tect_POS1	Tectum	QC
SA354947	Pooled_QC1_MS2_Tect_POS2	Tectum	QC
SA354948	Pooled_QC1_MS2_Tect_NEG2	Tectum	QC
SA354949	Pooled_QC2_MS1_Tect_NEG2	Tectum	QC
SA354950	Pooled_QC2_MS1_Tect_POS2	Tectum	QC
SA354951	Pooled_QC2_MS1_Tect_NEG1	Tectum	QC
SA354952	Pooled_QC2_MS2_Tect_POS1	Tectum	QC
SA354953	Pooled_QC2_MS2_Tect_POS2	Tectum	QC
SA354954	Pooled_QC2_MS2_Tect_NEG1	Tectum	QC
SA354955	Pooled_QC2_MS2_Tect_NEG2	Tectum	QC
SA354956	Pooled_QC1_MS1_Tect_NEG2	Tectum	QC
SA354957	Pooled_QC1_MS2_Tect_NEG1	Tectum	QC
SA354958	Pooled_QC1_MS1_Tect_POS2	Tectum	QC
SA354959	Pooled_QC1_MS1_Tect_POS1	Tectum	QC
SA354960	Pooled_QC1_MS1_Tect_NEG1	Tectum	QC
SA354961	Left_Tect_SHAM2_NEG2	Tectum	Sham
SA354962	Right_Tect_SHAM1_POS3	Tectum	Sham
SA354963	Right_Tect_SHAM2_NEG3	Tectum	Sham
SA354964	Right_Tect_SHAM2_NEG2	Tectum	Sham
SA354965	Right_Tect_SHAM2_NEG1	Tectum	Sham
SA354966	Right_Tect_SHAM2_POS3	Tectum	Sham
SA354967	Right_Tect_SHAM2_POS2	Tectum	Sham
SA354968	Right_Tect_SHAM2_POS1	Tectum	Sham
SA354969	Right_Tect_SHAM1_NEG3	Tectum	Sham
SA354970	Right_Tect_SHAM1_NEG2	Tectum	Sham
SA354971	Right_Tect_SHAM1_NEG1	Tectum	Sham
SA354972	Right_Tect_SHAM1_POS2	Tectum	Sham
SA354973	Left_Tect_SHAM2_NEG1	Tectum	Sham
SA354974	Right_Tect_SHAM1_POS1	Tectum	Sham
SA354975	Left_Tect_SHAM2_NEG3	Tectum	Sham
SA354976	Left_Tect_SHAM1_POS2	Tectum	Sham
SA354977	Left_Tect_SHAM1_POS3	Tectum	Sham
SA354978	Left_Tect_SHAM1_NEG1	Tectum	Sham
SA354979	Left_Tect_SHAM1_NEG2	Tectum	Sham
SA354980	Left_Tect_SHAM1_NEG3	Tectum	Sham
SA354981	Left_Tect_SHAM2_POS1	Tectum	Sham
SA354982	Left_Tect_SHAM2_POS2	Tectum	Sham
SA354983	Left_Tect_SHAM2_POS3	Tectum	Sham
SA354984	Left_Tect_SHAM1_POS1	Tectum	Sham

Showing results 1 to 100 of 100

Showing results 1 to 100 of 100

Collection:

Collection ID:	CO003392
Collection Summary:	The tissue was removed via dissection from the optic nerve head to the optic chiasm. The tecta were collected at 12- and 27-days post crush and separated into biological samples. Due to the small tissue and metabolomics resolution constraints, tissues were pooled to generate higher signal intensities. A total of 3 tecta were pooled into one tube.
Sample Type:	Eye tissue

Treatment:

Treatment ID:	TR003408
Treatment Summary:	Optic nerves from each transgenic Tg(Islet2b:EGFP-RPL10a) Xenopus laevis frogs, 3.5 - 5.0 cm in length, underwent monocular surgery of either a left optic crush injury (crush) or sham surgery (sham). The matching controls of uninjured right optic nerves were also collected (control). Operated individuals were anesthetized with 0.05% ethyl 3-aminobenzoate methanesulfonate (Sigma, USA).

Sample Preparation:

Sampleprep ID:	SP003406
Sampleprep Summary:	Tecta remained on dry ice to prevent metabolite degradation while the metabolite extraction was conducted. Tissues were transferred to 0.5mL Soft Tissue Lysing Kit Precellys tubes containing beads. Then, 84 µL of chilled 1:1 MeOH/H2O were added to Precellys tube. Pre-extraction internal standards were added to the tubes: 5µl of 1mg/ml Caffeine 13C6, 5µl of 1mg/ml D-Glucose 13C6, 5µl of 1mg/ml Oleic Acid 13C5, and 1µl of 5mg/mL Isoleucine 13C6 to each sample. Tissues were homogenized using Precellys 24 Touch. Cycle parameters: 2 cycles: 30 seconds homogenization at 4500 rpm, 10 seconds rest. Homogenate was transferred to a microcentrifuge tube and centrifuged at 18000xrcf for 20 min at 4°C. Then, collect supernatant and transfer pellet to Precellys Lysing Kit tube. Add 84uL of 8:1:1 Acetonitrile/Methanol/Acetone to pellet and add the rest of the pre-extraction internal standards: 5µl of 1mg/ml Caffeine 13C6, 5µl of 1mg/ml D-Glucose 13C6, 5µl of 1mg/ml Oleic Acid 13C5, 1µl of 5mg/mL Isoleucine 13C6. Final pre-extraction internal standards concentrations are 50μg/mL. Homogenization cycles were repeating using Precellys 24 Touch. Centrifuge as before and add second supernatant to first round of collected supernatant. Centrifuge at 1800xrcf for 20 min once more to remove any remaining tissue debris. Collect supernatant and dry supernatant in Speedvac. Two extraction blanks were prepared in the same manner as the biological samples. Dried samples were reconstituted immediately in 0.1% formic acid in 44.75µL of HPLC-MS grade water. Post-extraction internal standards were added: 25 µl of 5mg/ml Phenylalanine 13C6, 2.5 µl of .5mg/ml Uracil 13C 15N2, 1.25 µl of 1mg/ml Arginine 13C6, 1.25 µl of 1mg/ml Serine 13C3 to each sample.

Sampleprep ID:

SP003406

Sampleprep Summary:

Tecta remained on dry ice to prevent metabolite degradation while the metabolite extraction was conducted. Tissues were transferred to 0.5mL Soft Tissue Lysing Kit Precellys tubes containing beads. Then, 84 µL of chilled 1:1 MeOH/H2O were added to Precellys tube. Pre-extraction internal standards were added to the tubes: 5µl of 1mg/ml Caffeine 13C6, 5µl of 1mg/ml D-Glucose 13C6, 5µl of 1mg/ml Oleic Acid 13C5, and 1µl of 5mg/mL Isoleucine 13C6 to each sample. Tissues were homogenized using Precellys 24 Touch. Cycle parameters: 2 cycles: 30 seconds homogenization at 4500 rpm, 10 seconds rest. Homogenate was transferred to a microcentrifuge tube and centrifuged at 18000xrcf for 20 min at 4°C. Then, collect supernatant and transfer pellet to Precellys Lysing Kit tube. Add 84uL of 8:1:1 Acetonitrile/Methanol/Acetone to pellet and add the rest of the pre-extraction internal standards: 5µl of 1mg/ml Caffeine 13C6, 5µl of 1mg/ml D-Glucose 13C6, 5µl of 1mg/ml Oleic Acid 13C5, 1µl of 5mg/mL Isoleucine 13C6. Final pre-extraction internal standards concentrations are 50μg/mL. Homogenization cycles were repeating using Precellys 24 Touch. Centrifuge as before and add second supernatant to first round of collected supernatant. Centrifuge at 1800xrcf for 20 min once more to remove any remaining tissue debris. Collect supernatant and dry supernatant in Speedvac. Two extraction blanks were prepared in the same manner as the biological samples. Dried samples were reconstituted immediately in 0.1% formic acid in 44.75µL of HPLC-MS grade water. Post-extraction internal standards were added: 25 µl of 5mg/ml Phenylalanine 13C6, 2.5 µl of .5mg/ml Uracil 13C 15N2, 1.25 µl of 1mg/ml Arginine 13C6, 1.25 µl of 1mg/ml Serine 13C3 to each sample.

Combined analysis:

Analysis ID	AN005371	AN005372
Analysis type	MS	MS
Chromatography type	HILIC	HILIC
Chromatography system	Thermo Vanquish	Thermo Vanquish
Column	Thermo Accucore Amide HILIC (150 x 2.1mm, 2.6um)	Thermo Accucore Amide HILIC (150 x 2.1mm, 2.6um)
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:	CH004070
Chromatography Summary:	Positive ion mode
Instrument Name:	Thermo Vanquish
Column Name:	Thermo Accucore Amide HILIC (150 x 2.1mm, 2.6um)
Column Temperature:	35 C
Flow Gradient:	The gradient began at 1.0% B for 1 min, then shifted to 95.0% B for 9 minutes, then stayed at 95.0% B for 1 min before ramping down quickly to 1.0% B for 5 minutes.
Flow Rate:	0.5 ml/min
Solvent A:	95% acetonitrile/5% water/10mM Ammonium Formate/0.1% formic acid; 95% acetonitrile/5% water/10mM Ammonium Acetate/0.1% acetic acid
Solvent B:	50% acetonitrile/50% water/10mM Ammonium Formate/0.1% formic acid
Chromatography Type:	HILIC

Chromatography ID:	CH004071
Chromatography Summary:	Negative ion mode
Instrument Name:	Thermo Vanquish
Column Name:	Thermo Accucore Amide HILIC (150 x 2.1mm, 2.6um)
Column Temperature:	35 C
Flow Gradient:	The gradient began at 1.0% B for 1 min, then shifted to 95.0% B for 9 minutes, then stayed at 95.0% B for 1 min before ramping down quickly to 1.0% B for 5 minutes.
Flow Rate:	0.5 ml/min
Solvent A:	95% acetonitrile/5% water; 10mM Ammonium Acetate; 0.1% acetic acid
Solvent B:	50% acetonitrile/50% water; 10mM Ammonium Acetate; 0.1% acetic acid
Chromatography Type:	HILIC

MS:

MS ID:	MS005100
Analysis ID:	AN005371
Instrument Name:	Thermo Q Exactive Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	The samples were run using a Q ExactiveTM mass spectrometer coupled to a heated electrospray ionization (HESI) source. The spray voltage was set to 3.50 kV, capillary temperature to 350°C, sheath gas to 55, aux gas to 14, sweep gas to 4, and S-Lens RF Level to 30.0. The mass range was set to 67 – 1000 m/z, resolution 140,000 for full scan and 35,000 for ddMS2. AGC target was set to 1e6 for full scan and 2e5 for ddMS2. The max injection time (IT) was 100 seconds for full scan mode and 50 seconds for ddMS2. The number of microscans was 2, and normalized collision energy (NCE) was set to 20, 35, and 50. Samples were run in both positive and negative ion mode separately. The parameters for negative mode were the same except the spray voltage, which was set to 2.50 kV and capillary temperature to 380°C. Metabolites were identified from their Thermo.RAW scans using Compound DiscovererTM 3.3 software. Extraction blanks were used to determine and correct for reagent effects, allow for the creation of exclusions lists, mark background components, and filters the background components from the results table in Compound DiscovererTM 3.3. Pooled QCs were used for initial compound normalization and identification. All non-identified compounds were removed.
Ion Mode:	POSITIVE

MS ID:	MS005101
Analysis ID:	AN005372
Instrument Name:	Thermo Q Exactive Orbitrap
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	The samples were run using a Q ExactiveTM mass spectrometer coupled to a heated electrospray ionization (HESI) source. The spray voltage was set to 3.50 kV, capillary temperature to 350°C, sheath gas to 55, aux gas to 14, sweep gas to 4, and S-Lens RF Level to 30.0. The mass range was set to 67 – 1000 m/z, resolution 140,000 for full scan and 35,000 for ddMS2. AGC target was set to 1e6 for full scan and 2e5 for ddMS2. The max injection time (IT) was 100 seconds for full scan mode and 50 seconds for ddMS2. The number of microscans was 2, and normalized collision energy (NCE) was set to 20, 35, and 50. Samples were run in both positive and negative ion mode separately. The parameters for negative mode were the same except the spray voltage, which was set to 2.50 kV and capillary temperature to 380°C. Metabolites were identified from their Thermo.RAW scans using Compound DiscovererTM 3.3 software. Extraction blanks were used to determine and correct for reagent effects, allow for the creation of exclusions lists, mark background components, and filters the background components from the results table in Compound DiscovererTM 3.3. Pooled QCs were used for initial compound normalization and identification. All non-identified compounds were removed.
Ion Mode:	NEGATIVE