Detection of characteristic peptides of rat cyp2e1 enzyme and its screening method and application
A technology of characteristic peptides and peptides, which is applied in the field of biological detection and proteins, can solve the problems of high quantitative lower limit, insufficient sensitivity, and lack of method verification, and achieve the effect of high sensitivity, strong specificity, and avoiding interference
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Embodiment 1
[0045] This embodiment provides characteristic peptides for detecting rat CYP2E1 enzymes. The characteristic peptides include quantitative peptides, labeled peptides and extended peptides; the quantitative peptides include the first quantitative peptide and the second quantitative peptide. The amino acid sequences of the quantitative peptide and the second quantitative peptide are shown in SEQ ID NO.1-2; the labeled peptide includes the first labeled peptide and the second labeled peptide, the first labeled peptide and the second labeled peptide It is isotope labeling; the extended peptide segment includes a first extended peptide segment and a second extended peptide segment, and the amino acid sequences of the first extended peptide segment and the second extended peptide segment are shown in SEQ ID NO.3-4.
[0046] The isotope labeling method of the first labeled peptide is: FINL( 13 C 6 15 N 1 )VPSNLPHEATR; the isotope labeling mode of the second labeled peptide is GII(...
Embodiment 2
[0049] This embodiment provides a screening method for detecting characteristic peptides of rat CYP2E1 enzymes, comprising the following steps:
[0050] First, according to the amino acid sequence of the CYP2E1 enzyme, the digestion is simulated by Skyline software, and the length of the peptide segment for the simulation digestion is set to be 7-22 amino acids in length. Obtain the simulated enzyme-cleaved peptides, and obtain the ion information of each peptide; then use Uniprot software to exclude regions that do not conform to the characteristic peptides, such as metal binding sites, conflicting sequences, and post-translational modification sites. The Protein BLAST tool of NCBI database (http: / / blast.ncbi.nlm.nih.gov / Blast.cgi) can specifically identify candidate peptides. Input the protein or peptide sequence, select Rattusnorvegicus as the species, and analyze whether the two peptides meet the specificity requirements.
[0051] Secondly, the mouse liver microsome sampl...
Embodiment 3
[0065] This embodiment provides a screening method for detecting characteristic peptides of rat CYP2E1 enzymes, comprising the following steps:
[0066] First, according to the amino acid sequence of the CYP2E1 enzyme, the digestion is simulated by Skyline software, and the length of the peptide segment for the simulation digestion is set to be 7-22 amino acids in length. Obtain the simulated enzyme-cleaved peptides, and obtain the ion information of each peptide; then use Uniprot software to exclude regions that do not conform to the characteristic peptides, such as metal binding sites, conflicting sequences, and post-translational modification sites. The Protein BLAST tool of NCBI database (http: / / blast.ncbi.nlm.nih.gov / Blast.cgi) can specifically identify candidate peptides. Input the protein or peptide sequence, select Rattusnorvegicus as the species, and analyze whether the two peptides meet the specificity requirements.
[0067] Secondly, the mouse liver microsome sampl...
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