{
"METABOLOMICS WORKBENCH":{"STUDY_ID":"ST001721","ANALYSIS_ID":"AN002804","VERSION":"1","CREATED_ON":"March 15, 2021, 12:03 pm"},

"PROJECT":{"PROJECT_TITLE":"Detecting sex-related changes to the metabolome of a critically endangered freshwater crayfish during the mating season","PROJECT_TYPE":"MS analysis of crustacean haemolymph","PROJECT_SUMMARY":"Captive breeding is a vital tool in the conservation of highly endangered species, as it is for the Margaret River hairy marron, Cherax tenuimanus, from the south west of Australia. A close relative, Cherax cainii, has almost completely displaced C. tenuimanus in the wild and is a successful aquaculture species, whereas C. tenuimanus has performed poorly in captivity. We used untargeted liquid chromatography-mass spectrometry to obtain metabolomic profiles of female and male C. tenuimanus held in controlled aquarium conditions during their reproductive period. Using repeated haemolymph sampling we tracked the metabolomic profiles of animals just prior to and for a period of up to 34 days after pairing with a similar sized potential mate. We identified 54 reproducible annotated metabolites including amino acids, fatty acids, biogenic amines, purine and pyrimidine metabolites and excretion metabolites. Hierarchical clustering analysis distinguished five metabolite clusters. Principal component-canonical variate analysis clearly distinguished females from males, both unpaired and paired; similar trends in profile changes in both sexes after pairing; and a striking shift in males upon pairing. We discuss three main patterns of metabolomic responses: differentiation between sexes; reactive responses to the disturbance of pairing; and convergent response to the disturbance of pairing for males. Females generally had higher concentrations of metabolites involved in metabolic rate, mobilisation of energy stores and stress. Responses to the disturbance of pairing were also related to elevated stress. Females were mobilising lipid stores to deposit yolk, whereas males had a rapid and strong response to pairing, with shifts in metabolites associated with gonad development and communication, indicating males could complete reproductive readiness only once paired with a female. The metabolomic profiles support a previously proposed potential mechanism for displacement of C. tenuimanus by C. cainii in the wild and identify several biomarkers for testing hypotheses regarding reproductive success using targeted metabolomics.","INSTITUTE":"Edith Cowan University","DEPARTMENT":"School of Science","LAST_NAME":"Lette","FIRST_NAME":"Emily","ADDRESS":"270 Joondalup Drive, Joondalup, WA, 6027, Australia","EMAIL":"e.lette@ecu.edu.au","PHONE":"+61 8 6304 5513"},

"STUDY":{"STUDY_TITLE":"Detecting sex-related changes to the metabolome of a critically endangered freshwater crayfish during the mating season","STUDY_TYPE":"LC-MS analysis of crustacean haemolymph","STUDY_SUMMARY":"Captive breeding is a vital tool in the conservation of highly endangered species, as it is for the Margaret River hairy marron, Cherax tenuimanus, from the south west of Australia. A close relative, Cherax cainii, has almost completely displaced C. tenuimanus in the wild and is a successful aquaculture species, whereas C. tenuimanus has performed poorly in captivity. We used untargeted liquid chromatography-mass spectrometry to obtain metabolomic profiles of female and male C. tenuimanus held in controlled aquarium conditions during their reproductive period. Using repeated haemolymph sampling we tracked the metabolomic profiles of animals just prior to and for a period of up to 34 days after pairing with a similar sized potential mate. We identified 54 reproducible annotated metabolites including amino acids, fatty acids, biogenic amines, purine and pyrimidine metabolites and excretion metabolites. Hierarchical clustering analysis distinguished five metabolite clusters. Principal component-canonical variate analysis clearly distinguished females from males, both unpaired and paired; similar trends in profile changes in both sexes after pairing; and a striking shift in males upon pairing. We discuss three main patterns of metabolomic responses: differentiation between sexes; reactive responses to the disturbance of pairing; and convergent response to the disturbance of pairing for males. Females generally had higher concentrations of metabolites involved in metabolic rate, mobilisation of energy stores and stress. Responses to the disturbance of pairing were also related to elevated stress. Females were mobilising lipid stores to deposit yolk, whereas males had a rapid and strong response to pairing, with shifts in metabolites associated with gonad development and communication, indicating males could complete reproductive readiness only once paired with a female. The metabolomic profiles support a previously proposed potential mechanism for displacement of C. tenuimanus by C. cainii in the wild and identify several biomarkers for testing hypotheses regarding reproductive success using targeted metabolomics.","INSTITUTE":"Edith Cowan University","DEPARTMENT":"School of Science","LAST_NAME":"Lette","FIRST_NAME":"Emily","ADDRESS":"270 Joondalup Drive, Joondalup, WA, 6027, Australia","EMAIL":"e.lette@ecu.edu.au","PHONE":"+61 8 6304 5513","TOTAL_SUBJECTS":"10","NUM_MALES":"5","NUM_FEMALES":"5"},

"SUBJECT":{"SUBJECT_TYPE":"Invertebrate","SUBJECT_SPECIES":"Cherax tenuimanus","TAXONOMY_ID":"99755","WEIGHT_OR_WEIGHT_RANGE":"116g-198g","GENDER":"Male and female"},
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],
"COLLECTION":{"COLLECTION_SUMMARY":"All haemolymph collections for all animals occurred at the same time of day and the animals were handled in the same order on each of the four collection dates. Haemolymph (200mL) was extracted from the ventral sinus of each crayfish using a 21G needle and 1mL syringe inserted into the soft tissue at the base of the 5th pereopod. Haemolymph was added to 2mL Eppendorf tubes preloaded with 600µL LC-MS grade acetonitrile (Optima, Thermo Fisher Scientific, AUS) containing deuterated internal standards (d8- valine, d9 –trimethylamine-N-oxide (TMAO) , d3-leucine, d6-trans-cinnamic acid, d5-tryptophan, 1g/mL) from Cambridge Isotope Laboratories (Cambridge, MA, USA) and stored on ice. Samples were mixed at 1400rpm (Thermal Mixer, Thermo Fisher Scientific, AUS) for 60 seconds at 4°C, then centrifuged (Heraeus Megafuge 8R, Thermo Fisher Scientific, AUS) for 20 minutes (1800  g) at 4°C. After centrifuging, 100µL of supernatant was aliquoted into five separate vials. The samples were then dried using a SpeedVac centrifugal vacuum concentrator (Thermo Fisher Scientific, AUS). The dried samples were stored at -80°C for subsequent metabolomics analysis.","COLLECTION_PROTOCOL_FILENAME":"EmilyLette_20210225_014138_PR_CO_Methods__Lette_marron.pdf","SAMPLE_TYPE":"Hemolymph","COLLECTION_METHOD":"aspiration","COLLECTION_LOCATION":"ventral sinus accessed from soft tissue at base of 5th pereopod","STORAGE_CONDITIONS":"-80℃","COLLECTION_VIALS":"2mL Eppendorf tubes","STORAGE_VIALS":"2mL Eppendorf tubes"},

"TREATMENT":{"TREATMENT_SUMMARY":"Cherax tenuimanus (n=10) were housed in aquaria as individuals prior to sampling at timepoint 1. After timepoint 1 they were placed in pairs with a potential mate of the opposite sex and housed in aquaria over the next four weeks which included timepoints 2-4."},

"SAMPLEPREP":{"SAMPLEPREP_SUMMARY":"The dried haemolymph samples were reconstituted using 100µL of LC-MS water containing 0.1% Formic acid. Samples were manually swirled, then placed in a thermomixer for 2 minutes at 4oC, before being centrifuged at (1800  g) for 5 minutes at 4oC. Next, 40µL of the supernatant was transferred into LC-MS amber vials with inserts and placed in the autosampler kept at 6oC. The order in which samples were analysed was randomised to avoid any potential instrument bias. A pooled quality control (QC) sample was prepared by adding 40 µL from each reconstituted sample to a single Eppendorf tube, which was then mixed to homogenise in a thermal mixer and centrifuged as above. This pooled sample was aliquoted (40µL) into LC-MS amber vials to create 16 QC samples and placed into the autosampler tray kept at 6°C ready for analysis. Samples were analysed within 24 hours from preparation. At the start of the analytical batch, a solvent blank, matrix blank, and ten conditioning QC samples were analysed (Broadhurst et al., 2018). QC samples were then injected after every fifth marron haemolymph sample with two QCs analysed at the end of the batch, following the standard protocols for metabolomics (Broadhurst et al., 2018).","PROCESSING_STORAGE_CONDITIONS":"Described in summary"},

"CHROMATOGRAPHY":{"CHROMATOGRAPHY_TYPE":"Reversed phase","INSTRUMENT_NAME":"Thermo Dionex Ultimate 3000 RS","COLUMN_NAME":"Thermo Hypersil GOLD C18 (100 x 2.1mm,1.9µm)","FLOW_GRADIENT":"isocratic at 99% A: 1 min; 50% B:1-2 min; linear increase to 99% B: over 7min; 99% B: 2min; initial conditions returned over 2 min; 100% A: 3 min.","FLOW_RATE":"0.3mL/min","COLUMN_TEMPERATURE":"45","METHODS_FILENAME":"Methods_Lette_marron","SOLVENT_A":"0.1% formic acid in LC-MS water","SOLVENT_B":"0.1% formic acid in LC-MS acetonitrile"},

"ANALYSIS":{"ANALYSIS_TYPE":"MS","ANALYSIS_PROTOCOL_FILE":"Methods_Lette_marron"},

"MS":{"INSTRUMENT_NAME":"Thermo Q Exactive Orbitrap","INSTRUMENT_TYPE":"Orbitrap","MS_TYPE":"ESI","ION_MODE":"POSITIVE","MS_COMMENTS":"Full scans with data-dependent tandem mass spectrometry were acquired on the Orbitrap mass analyzer. Full scans were acquired at a resolution of 70,000 at mass-to-charge ratio (m/z) 200 over the m/z range 70–1000 with the ESI conditions as follows: source heater = 350°C, sheath gas = 35 (arbitrary units), auxiliary gas = 10 (arbitrary units), capillary temperature 350°C, ion spray voltage = 3.0 kV (positive ion mode) and 2.5 kV (negative ion mode), S-lens 50%, and automatic gain control = 110¬¬¬-6. Tandem mass spectrometry experiments were performed at a resolution of 17,500 at m/z 200 on each sample with the higher energy collisional dissociation energy set at 20 eV. Data acquisition was carried out using Xcalibur software (Thermo Fisher Scientific). Before analysis, the Orbitrap was externally calibrated using ready-made calibration solutions (ESI-negative ion calibration and ESI-positive ion calibration solutions) obtained from Thermo Fisher Scientific."},

"MS_METABOLITE_DATA":{
"Units":"peak area values",

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"Metabolites":[{"Metabolite":"2-Piperidinone","KEGG ID":"-","PubChem ID":"12665","Formula":"C5 H9 N O","retention time":"3.038","MW":"99.06876"},{"Metabolite":"Carnitine","KEGG ID":"C00318","PubChem ID":"10917","Formula":"C7 H15 N O3","retention time":"0.886","MW":"161.10516"},{"Metabolite":"Thymine","KEGG ID":"C00178","PubChem ID":"1135","Formula":"C5 H6 N2 O2","retention time":"2.97","MW":"126.04304"},{"Metabolite":"Betaine","KEGG ID":"C00719","PubChem ID":"248","Formula":"C5 H11 N O2","retention time":"0.866","MW":"117.07913"},{"Metabolite":"CAR 2:0","KEGG ID":"C002571","PubChem ID":"7045767","Formula":"C9 H17 N O4","retention time":"1.293","MW":"203.11579"},{"Metabolite":"Kynurenic acid","KEGG ID":"C01717","PubChem ID":"3845","Formula":"C10 H7 N O3","retention time":"3.226","MW":"189.04259"},{"Metabolite":"Tyrosine","KEGG ID":"C00082","PubChem ID":"6057","Formula":"C9 H11 N O3","retention time":"1.668","MW":"181.07394"},{"Metabolite":"Kynurenine","KEGG ID":"C00328","PubChem 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}

}