Abstract

Background:Snail (Oncomelania hupensis) control is an important and effective preventive strategy in schistosomiasis control programs, and screening microbial molluscicidal agents is one of the most promising categories in biomolluscicides.Objective:To purify and identify the molluscicidal ingredient (MI) obtained from strain SL-30's exocellular broth.Materials and Methods:The active extracts extracted from SL-30's exocellular broth was purified on a silica gel column guided by molluscicidal activity assay against Oncomelania hupensis, then the MI was obtained. NMR spectroscopy and LC-MS/MS analysis was used to identify the molecular structure of the MI.Results:Molluscicidal activity bioassay showed that the MI exhibited significant molluscicidal activity with the LC50 values of 0.101, 0.062, and 0.022 mg/L, respectively, in the case of exposure period of 24 h. From 1H NMR, 13C NMR, 1H-1H COSY, and 1H-13C HSQC spectra, partial important structure fragment was obtained, and the relative molecular weight of the MI showed 326 according to LC-MS analysis. Then, on these grounds, it was indicated that the molecular structure of the MI had a higher similarity to Gliotoxin with the molecular formula of C13 H14N2O4S2. The quasi-molecular ion of m/z 325.45 was further analyzed by MS2 as the parent ion, and two daughter ions obtained at m/z 295.11 [M-CH2OH]- and m/z 261.08 [M-CH2OH -2S]–Conclusion:The MI was finally confirmed as Gliotoxin.

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