Underivatized polyamine analysis in plant samples by ion pair LC coupled with electrospray tandem mass spectrometry |
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Authors: | Jose Sánchez-López Gemma Camañes Víctor Flors Cristian Vicent Victoria Pastor Begonya Vicedo Miguel Cerezo Pilar García-Agustín |
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Affiliation: | 1. Key Laboratory of Nature Resource of Changbai Mountain and Functional Molecular (Yanbian University), Ministry of Education, Yanji 133002, China;2. Department of Chemistry, Changwon University, Changwon 641-773, Republic of Korea;1. Department of Biotechnology, GITAM Institute of Science, GITAM University, Visakhapatnam 530 045, Andhra Pradesh, India;2. Department of Biochemistry, GITAM Institute of Science, GITAM University, Visakhapatnam 530 045, Andhra Pradesh, India;3. Scientist–Biocare, Centre for DNA Fingerprinting and Diagnostics, Hyderabad, Telangana, India |
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Abstract: | Polyamines are key regulators of cell development and many plant responses to environmental challenges, however, their functions still remain unclear in complex interactions with other hormones and in biotic or abiotic stress. This lack of knowledge derives from the difficulties on measuring natural polyamines in plants. Here, we present a fast multiresidue method for putrescine (Put), 1,3-diaminopropane (DAP), l-ornithine, spermidine (Spd) and spermine (Spn) measurements in plant samples. Polyamine determination is based on a perchloric acid extraction followed by a simple filtration procedure without previous derivatization. Polyamines are resolved by HPLC in a C18 common column and quantified by electrospray ionization tandem mass spectrometry. 13C4-putrescine and 1,7-diaminoheptane standards were added prior to sample extraction to achieve an accurate quantification in a single run. Chromatography of polyamines presents poor retention when reverse phase C18 common columns are used, because they are very polar compounds and contain several positive charges. To circumvent this problem ionic pairing technique has been used successfully with heptafluorobutyric acid (HFBA) at 1 mM in the aqueous phase and 25 mM in the sample. Improvement of the signal depleted by HFBA has been achieved by adding 1% of propionic acid to the aqueous and organic eluents. All together, gives a method accurate enough to determine polyamines in plants. To demonstrate the usefulness of the method it has been validated in Arabidopsis thaliana samples and polyamines have been determined in several genotypes that over express (35S::ADC2 line 3.6) or are disrupted (adc2) in the Arginine Decarboxylase2 (ADC2) gene. |
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