Reduction of Membrane Lipid Metabolism in Postharvest Hami Melon Fruits by n-Butanol to Mitigate Chilling Injury and the Cloning of Phospholipase D-β Gene
Abstract
:1. Introduction
2. Materials and Methods
2.1. Materials and Reagents
2.2. Instruments and Equipment
2.3. Methods
2.3.1. Sample Handling
2.3.2. Determination of the Chilling Injury Index
2.3.3. Determination of Cell Membrane Permeability
2.3.4. Determination of MDA Content
2.3.5. Determination of the Contents of PI and PA
2.3.6. Determination of the Contents of Fatty Acids
2.3.7. Assay of LOX
- (1)
- Preparation of reaction substrate: The enzyme reaction substrate used in the test was 10 mmol/L sodium linoleate, and the amount of 70 mg sodium linoleate, 70 mLTriton X-100, and 4 mL anaerobic water were mixed (to avoid bubbles). After titration with 0.5 mol/L sodium hydroxide, the solution was clarified, the volume was 25 mL, and the volume was divided into 1.0–1.5 mL and stored at −18 °C until use.
- (2)
- Extraction of crude enzyme solution: 2.0 g of pulp tissue was placed in a mortar, ground with liquid nitrogen, added with 10 mL of 50 mmol/L (pH 7.0) phosphate buffer precooled at 4 °C, centrifuged at 15,000× g (4 °C) for 15 min, and the supernatant was used for LOX activity determination.
- (3)
- Determination of enzyme activity: the reaction system of 3 mL contained 25 μL sodium linoleate mother liquor, 2.775 mL buffer, and 0.2 mL enzyme solution, and the reaction temperature was 30 °C. The LOX activity was measured at 234 nm. The timing began 15 s after adding the enzyme solution, and the OD value change was recorded within 1 min. The enzyme activity was measured as ∆OD234/gFW·min. The procedure was repeated 3 times.
2.3.8. Assay of PLD
2.3.9. RNA Extraction, cDNA Synthesis, and Primer Analysis by Quantitative Fluorescent PCR (Q-PCR)
2.3.10. Gene Cloning
2.3.11. Data Processing and Analysis
3. Results
3.1. Effects of n-Butanol Treatment on Chilling Injury Symptoms and Chilling Injury Index of Hami Melon Fruits during Storage
3.2. Effect of n-Butanol on Cell Membrane Permeability and the MDA Content of Hami Melon
3.3. Effect of n-Butanol on the PI and PA Contents of Hami Melon
3.4. Effect of n-Butanol on Saturated Fatty Acid Content of Hami Melon
3.5. Effect of n-Butanol on the Unsaturated Fatty Acid Content of Hami Melon
3.6. Effect of n-Butanol on LOX Activity and CmLOX Expression in Hami Melon
3.7. Effect of n-Butanol on PLD Activity and CmPLD-β Expression in Hami Melon
3.8. Sequence Analysis of the Hami Melon PLD-β Gene
3.8.1. Evolutionary Tree Analysis of the Base Sequence Homology of Hami Melon Rind PLD-β Gene with Multiple Species
3.8.2. Evolutionary Tree Analysis of Nucleic Acid Sequence Homology of PLD-β Gene in Hami Melon Pericarp with Multiple Species
3.8.3. Twofold Comparison of the CmPLD-β Gene and Target Gene in Hami Melon Pericarp
4. Discussion
5. Conclusions
Author Contributions
Funding
Data Availability Statement
Conflicts of Interest
References
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Instrument Name | Instrument Model | Instrument Manufacturers |
---|---|---|
Nitrogen purge instrument | Thermo | Reacti-thermo (MA, USA) |
Mass Spectrometer | Q Exactive (MA, USA) | |
UPLC | Vanquish (MA, USA) | |
Freeze dryer | Four rings | LGJ-10 (Beijing, China) |
Enzyme Markers | HBS-1101 | Nanjing Detie Test Equipment Co. (Nanjing, China) |
Category | Accession Number | Sequence (5′ to 3′) |
---|---|---|
CmPLD | CmPLD-F | CAGGCAGAGAATGAGAACAACA |
CmPLD-R | AGGGGATATGTGGATAATCCGT | |
CmLOX | CmLOX-F | GCACAACACGCAGCACTAAA |
CmLOX-R | CTCTGGA TCGTTCTCGTCGG | |
18S | 18S-F | GCTGTCACTGTTTTTGGCGT |
18S-R | GCACCACCCTTCAAATGAGC |
Primer Name | Primer Sequences |
---|---|
PLD-F | ACCCATACCCTCGTCCAATTCCATCTC |
PLD-R | TGTCCGTCTGGAACATGGGCATCTTG |
PLD-F | AGCCATGTAAGCCTGGAGCTGCTCTAAG |
PLD-R | TGAACTCCATAGGGTTACAAAGGCCACTC |
PLD-F | TCCATATCACAATCCTTACCCATACCCTC |
PLD-R | AGATAGTGAGGTTCTCCTGAATTCCAAG |
PLD-F | ACACACATGCATACATACTGTCGCTC |
PLD-R | ACTCCATAGGGTTACAAAGGCCACTC |
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Huang, S.; Bi, Y.; Li, H.; Liu, C.; Wang, X.; Wang, X.; Lei, Y.; Zhang, Q.; Wang, J. Reduction of Membrane Lipid Metabolism in Postharvest Hami Melon Fruits by n-Butanol to Mitigate Chilling Injury and the Cloning of Phospholipase D-β Gene. Foods 2023, 12, 1904. https://doi.org/10.3390/foods12091904
Huang S, Bi Y, Li H, Liu C, Wang X, Wang X, Lei Y, Zhang Q, Wang J. Reduction of Membrane Lipid Metabolism in Postharvest Hami Melon Fruits by n-Butanol to Mitigate Chilling Injury and the Cloning of Phospholipase D-β Gene. Foods. 2023; 12(9):1904. https://doi.org/10.3390/foods12091904
Chicago/Turabian StyleHuang, Shuai, Ying Bi, Hui Li, Caihong Liu, Xue Wang, Xinyu Wang, Yaxin Lei, Qi Zhang, and Jing Wang. 2023. "Reduction of Membrane Lipid Metabolism in Postharvest Hami Melon Fruits by n-Butanol to Mitigate Chilling Injury and the Cloning of Phospholipase D-β Gene" Foods 12, no. 9: 1904. https://doi.org/10.3390/foods12091904
APA StyleHuang, S., Bi, Y., Li, H., Liu, C., Wang, X., Wang, X., Lei, Y., Zhang, Q., & Wang, J. (2023). Reduction of Membrane Lipid Metabolism in Postharvest Hami Melon Fruits by n-Butanol to Mitigate Chilling Injury and the Cloning of Phospholipase D-β Gene. Foods, 12(9), 1904. https://doi.org/10.3390/foods12091904