Glucosinolate Analysis in Whole Rapeseed by Near Infrared Reflectance Spectroscopy

Renard, Michel; Bernard, C.; Deschamps, M.; Furtoss, Vincent; Lila, M.; Quinsac, Alain; Regnier, J. M.; Ribaillier, D.

doi:10.1007/978-94-009-3615-7_13

Cited by 10 publications

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“…NIRS calibrations for the analysis of total GSL content have been developed for Brassica napus and Brassica rapa (Renard et al 1987, Daun et al 1994, Brassica carinata (Velasco et al 1995), and Brassica juncea (A. De Haro, personal communication) because breeding for low GSL content has focused mainly on these species.…”

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“…These methods were designed to estimate the total GSL content, and do not provide simultaneous information on the GSL profile (Sorensen 1985). The development of near-infrared reflectance spectroscopy (NIRS) calibrations to estimate the total GSL content in intact seeds represented a further advance, since it could be estimated in parallel with the analysis of other traits such as oil and protein content (Renard et al 1987).NIRS calibrations for the analysis of total GSL content have been developed for Brassica napus and Brassica rapa (Renard et al 1987, Daun et al 1994, Brassica carinata (Velasco et al 1995), and Brassica juncea (A. De Haro, personal communication) because breeding for low GSL content has focused mainly on these species.…”

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Analysis of total glucosinolate content and individual glucosinolates in Brassica spp. by near‐infrared reflectance spectroscopy

Velasco¹,

Becker²

1998

Plant Breeding

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This study was conducted to test the applicability of near-infrared reflectance spectroscopy (NIRS) for estimating the total glucosinolate (GSL) content in samples of intact seed from a wide range of Brassica species, and to develop calibration equations to estimate simultaneously the percentage of individual GSLs. A total of 290 samples from 15 different Brassica species were scanned by NIRS and analysed for glucosinolate content by high-pressure liquid chromatography (HPLC). A calibration equation for total GSL content was developed using 270 samples of 14 species in a range between 6 and 193 /imol/g seed, resulting in an r^ of 0.99 in calibration and cross-validation, and 0.95 in independent validation with 20 samples of Brassica rapa, a species not represented in the calibration. Furthermore, calibration equations to estimate the relative amount (mol/mol) of progoitrin, sinigrin, and gluconapin were successfully developed (r^ > 0.85 in cross-validation) and validated with samples from species not included in the calibration. It was also possible to discriminate between entries with high and low values of glucoiberin, 4-hydroxyglucobrassicin and glucoerucin.Key words: Brassica spp. -individual glucosinolates -nearinfrared reflectance spectroscopy -NIRS -total glucosinolate content Breeding for low glucosinolate (GSL) content in Brassica oilseeds has been the subject of intensive research during recent decades because of the toxic and antinutritive effects of these compounds (Downey and Robbelen 1989). Success in this field was facihtated considerably by the development of rapid and accurate methods which permit large screenings to be made in a short time and at a low cost (Thies 1982). These methods were designed to estimate the total GSL content, and do not provide simultaneous information on the GSL profile (Sorensen 1985). The development of near-infrared reflectance spectroscopy (NIRS) calibrations to estimate the total GSL content in intact seeds represented a further advance, since it could be estimated in parallel with the analysis of other traits such as oil and protein content (Renard et al. 1987).NIRS calibrations for the analysis of total GSL content have been developed for Brassica napus and Brassica rapa (Renard et al. 1987, Daun et al. 1994, Brassica carinata (Velasco et al. 1995), and Brassica juncea (A. De Haro, personal communication) because breeding for low GSL content has focused mainly on these species. The use of this technique for the analysis of other Brassica species is now of great interest because of new research lines developed in recent years which involve alternative uses for glucosinolates, such as application in pest and disease control (Mithen 1992) or characterization as substances with anticancer activity (Giamoustaris and Mithen 1996). This will demand rapid analysis of GSLs in a wide range of Brassica species and it would be a very helpful analytical tool in interspecific breeding. The analysis of total GSL content in several Brassica species could be made possible by devel...

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Analysis of total glucosinolate content and individual glucosinolates in Brassica spp. by near‐infrared reflectance spectroscopy

Velasco¹,

Becker²

1998

Plant Breeding

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“…The glucose release methods (Van Etten et al 1974, Smith andDacombe 1987) based on a colorimetric glucose oxidase/peroxidase assay including the clinical glucose test paper (Tes-Tape) method for urine sugar (Lein 1970, McGregor andDowney 1975), and the TRUBLUGLU meter method (Tholen et al 1993), have since been developed. Palladium method (Thies 1982, Møller et al 1985 and nondestructive quality evaluation methods using X-ray fluorescence spectroscopy (Schnug and Haneklaus 1988) and near-infrared reflectance spectroscopy (Renard et al 1987, Biston et al 1988 have also been developed. Specific ELISA assays have been developed for the determination of sinigrin and progoitrin that are major glucosinolates in Brussels sprouts (Van Doorn et al 1998).…”

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Simple and Rapid Method for the Selection of Individual Rapeseed Plants Low in Glucosinolates

2003

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A simple and rapid colorimetric method for the selection of individual rapeseed plants with low glucosinolate contents was developed using one of a pair of germinated cotyledons of a single seedling and a glucose-measuring method employed in clinical tests (CII-Test method). The CII-Test method can be used to estimate the amount of glucose released by the hydrolysis of glucosinolates extracted from a germinated cotyledon. In the present experiment, HPLC analysis showed that the total glucosinolate content of germinated cotyledons was not significantly different from that of seeds three days after seed sowing. When the glucosinolate content of the seeds and/or cotyledons was estimated by the glucosemeasuring CII-Test method and HPLC method, high positive correlations were recognized between both types of measurements. The CII-Test method exhibits some clear advantages in that 1) the glucosinolate content can be estimated in an individual plant, and 2) 150-500 samples can be estimated by one person in one day. These advantages indicate that the glucose measuring CII-Test method is suitable for efficient and accurate selection of rapeseed plants with low glucosinolate contents in the F 2 generation.

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“…Methods that indicate the total amount of glucosinolates are often based on the measurement of released glucose (vanEtten et al, 1974;Thies, 1985;Fiebig and Kallweit, 1987) or bisulfate ions (Fiebig and Sendfeld, 1989;Sendfeld et al, 1988) by enzymatic assays. Other methods include the palladium test (Thies, 1982), the near-infrared method (Renard et al, 1987), and the X-ray fluorescence method Haneklaus, 1987, 1988;Haneklaus et al, 1994). Individual glucosinolates were determined directly by GLC analysis of the trimethylsilyl derivates of glucosinolates (Thies, 1976), HPLC analysis of the intact glucosinolates (Helboe et al, 1980), and HPLC analysis of desulfoglucosinolates (Minchinton et al, 1982;Spinks et al, 1984;Fiebig and Jo ¨rden, 1990) or indirectly by GLC analysis of the enzymatic hydrolysis products (Daxenbichler and vanEtten, 1977;vanEtten and Daxenbichler, 1977).…”

Section: Introductionmentioning

confidence: 99%

Simultaneous Determination of Isothiocyanates, Indoles, and Oxazolidinethiones in Myrosinase Digests of Rapeseeds and Rapeseed Meal by HPLC

Matthäus

Fiebig

1996

J. Agric. Food Chem.

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HPLC has been used for the analysis of isothiocyanates, indoles, and oxazolidinethiones in rapeseeds and rapeseed meal. The samples were treated with myrosinase and the released hydrolysis products extracted with dichloromethane. The separation was performed on an RP-18 column using a gradient system with acetonitrile and water. Use of a programmable UV detector permitted the detection of the compounds at their absorption maxima of 210 and 240 nm, respectively. Response factors of eight standard compounds were calculated for 240 nm. The contents of glucosinolates calculated with the results of this method showed a significant linear correlation (r = 0.9995; P < 0.005) with the contents of glucosinolates evaluated with the results of the HPLC method of desulfoglucosinolates. Keywords: HPLC; indoles; isothiocyanates; oxazolidinethiones; rapeseed

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Glucosinolate Analysis in Whole Rapeseed by Near Infrared Reflectance Spectroscopy

Cited by 10 publications

References 1 publication

Analysis of total glucosinolate content and individual glucosinolates in Brassica spp. by near‐infrared reflectance spectroscopy

Analysis of total glucosinolate content and individual glucosinolates in Brassica spp. by near‐infrared reflectance spectroscopy

Simple and Rapid Method for the Selection of Individual Rapeseed Plants Low in Glucosinolates

Simultaneous Determination of Isothiocyanates, Indoles, and Oxazolidinethiones in Myrosinase Digests of Rapeseeds and Rapeseed Meal by HPLC

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