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Genetic deletion of LOX-1 attenuates metabolic dysfunction-associated steatohepatitis in mice

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DataCite Commons2025-12-22 更新2026-05-05 收录
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Supplement table1:The DNA was extracted from the mouse tail and amplified by PCR. The PCR reaction system included DNA, primers, 2×Taq premix and ddH2O, and the amplified products were subjected to agarose gel electrophoresis for visualization and image acquisition. Primer sequences for PCR were listed in Supplement Table 1.Supplement table2:Total RNA was extracted from the liver tissues of mice or LX-2 cells using RNAquick Purification Kit (Shanghai Yishan Biotechnology, Shanghai, China) as described by the manufacturer. cDNA synthesis was carried out with HiScript Ⅱ Q Select RT SuperMix for qPCR (Vazyme). Quantitative PCR was performed in technical triplicates using SYBR Green reagent (Vazyme). The level of β-actin or GAPDH RNA expression was used to normalize the data. Primer sequences for RT-qPCR were listed in Supplement Table 2.Supplement table3:Gene functional annotation of LOX-1-related MASH targets.
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2025-12-22
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