TY  - JOUR
A1  - Sagu Tchewonpi, Sorel
A1  - Landgräber, Eva
A1  - Rackiewicz, Michal
A1  - Huschek, Gerd
A1  - Rawel, Harshadrai Manilal
T1  - Relative Abundance of Alpha-Amylase/Trypsin Inhibitors in Selected Sorghum Cultivars
JF  - Molecules
N2  - Sorghum is of growing interest and considered as a safe food for wheat related disorders. Besides the gluten, α-amylase/trypsin-inhibitors (ATIs) have been identified as probable candidates for these disorders. Several studies focused on wheat-ATIs although there is still a lack of data referring to the relative abundance of sorghum-ATIs. The objective of this work was therefore to contribute to the characterization of sorghum ATI profiles by targeted proteomics tools. Fifteen sorghum cultivars from different regions were investigated with raw proteins ranging from 7.9 to 17.0 g/100 g. Ammonium bicarbonate buffer in combination with urea was applied for protein extraction, with concentration from 0.588 ± 0.047 to 4.140 ± 0.066 mg/mL. Corresponding electrophoresis data showed different protein profiles. UniProtKB data base research reveals two sorghum ATIs, P81367 and P81368; both reviewed and a targeted LC–MS/MS method was developed to analyze these. Quantifier peptides ELAAVPSR (P81367) and TYMVR (P81368) were identified and retained as biomarkers for relative quantification. Different reducing and alkylating agents were assessed and combination of tris (2 carboxyethyl) phosphine/iodoacetamide gave the best response. Linearity was demonstrated for the quantifier peptides with standard recovery between 92.2 and 107.6%. Nine sorghum cultivars presented up to 60 times lower ATI contents as compared to wheat samples. This data suggests that sorghum can effectively be considered as a good alternative to wheat.
KW  - sorghum
KW  - α-amylase/trypsin inhibitors
KW  - reducing agents
KW  - cysteine alkylation
KW  - SDS PAGE
KW  - targeted proteomics
KW  - LC–MS/MS
Y1  - 2020
U6  - https://doi.org/10.3390/molecules25245982
SN  - 1420-3049
VL  - 25
IS  - 24
PB  - MDPI
CY  - Basel
ER  - 
TY  - JOUR
A1  - Chmielewski, Frank M.
A1  - Baldermann, Susanne
A1  - Götz, Klaus Peter
A1  - Homann, Thomas
A1  - Gödeke, Kristin
A1  - Schumacher, Fabian
A1  - Huschek, Gerd
A1  - Rawel, Harshadrai Manilal
T1  - Abscisic acid related metabolites in sweet cherry buds (Prunus avium L.)
JF  - Journal of Horticulture
N2  - As our climate changes, plant mechanisms involved for dormancy release become increasingly important for commercial orchards. It is generally believed that abscisic acid (ABA) is a key hormone that responds to various environmental stresses which affects bud dormancy. For this reason, a multi-year study was initiated to obtain data on plant metabolites during winter rest and ontogenetic development in sweet cherry buds (Prunus avium L.). In this paper, we report on metabolites involved in ABA synthesis and catabolism and its effect on bud dormancy in the years 2014/15-2016/17. In previous work, the timings of the different phases of para-, endo-, ecodormancy and ontogenetic development for cherry flower buds of the cultivar ‘Summit’ were determined, based on classical climate chamber experiments and changes in the bud’s water content. Based on these time phases, we focused now on the different aspects of the ABA-metabolism. The results show that there is a continual synthesis of ABA about 5 weeks before leaf fall, and a degradation of ABA during ecodormancy and bud development until the phenological stage ‘open cluster’. This is confirmed by relating the ABA content to that of the total precursor carotenoids, neoxanthin and violaxanthin. The tentative monitoring of individual intermediate metabolites revealed that dihydroxyphaseic acid is the most abundant catabolite of ABA and ABA glucosyl ester is in terms of mass intensity, the most abundant ABA metabolite observed in this study. The results suggest that the direct route for ABA biosynthesis from farnesyl pyrophosphate may also be relevant in cherry flower buds.
KW  - Dormancy
KW  - Abscisic acid
KW  - Synthesis
KW  - Catabolism
KW  - Prunus avium L.
KW  - Flower buds
Y1  - 2018
U6  - https://doi.org/10.4172/2376-0354.1000221
SN  - 2376-0354
VL  - 5
IS  - 1
ER  - 
TY  - GEN
A1  - Baldermann, Susanne
A1  - Homann, Thomas
A1  - Neugart, Susanne
A1  - Chmielewski, Frank M.
A1  - Götz, Klaus-Peter
A1  - Gödeke, Kristin
A1  - Huschek, Gerd
A1  - Morlock, Gertrud E.
A1  - Rawel, Harshadrai Manilal
T1  - Selected Plant Metabolites Involved in Oxidation-Reduction Processes during Bud Dormancy and Ontogenetic Development in Sweet Cherry Buds (Prunus avium L.)
T2  - Molecules
N2  - Many biochemical processes are involved in regulating the consecutive transition of different phases of dormancy in sweet cherry buds. An evaluation based on a metabolic approach has, as yet, only been partly addressed. The aim of this work, therefore, was to determine which plant metabolites could serve as biomarkers for the different transitions in sweet cherry buds. The focus here was on those metabolites involved in oxidation-reduction processes during bud dormancy, as determined by targeted and untargeted mass spectrometry-based methods. The metabolites addressed included phenolic compounds, ascorbate/dehydroascorbate, reducing sugars, carotenoids and chlorophylls. The results demonstrate that the content of phenolic compounds decrease until the end of endodormancy. After a long period of constancy until the end of ecodormancy, a final phase of further decrease followed up to the phenophase open cluster. The main phenolic compounds were caffeoylquinic acids, coumaroylquinic acids and catechins, as well as quercetin and kaempferol derivatives. The data also support the protective role of ascorbate and glutathione in the para- and endodormancy phases. Consistent trends in the content of reducing sugars can be elucidated for the different phenophases of dormancy, too. The untargeted approach with principle component analysis (PCA) clearly differentiates the different timings of dormancy giving further valuable information.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 467 
KW  - dormancy
KW  - redox-metabolites
KW  - phenolics
KW  - ascorbate
KW  - anti-oxidative capacity
KW  - Prunus avium L.
KW  - flower buds
Y1  - 2018
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-417442
ER  - 
TY  - JOUR
A1  - Baldermann, Susanne
A1  - Homann, Thomas
A1  - Neugart, Susanne
A1  - Chmielewski, Frank M.
A1  - Götz, Klaus-Peter
A1  - Gödeke, Kristin
A1  - Huschek, Gerd
A1  - Morlock, Gertrud E.
A1  - Rawel, Harshadrai Manilal
T1  - Selected Plant Metabolites Involved in Oxidation-Reduction Processes during Bud Dormancy and Ontogenetic Development in Sweet Cherry Buds (Prunus avium L.)
JF  - Molecules
N2  - Many biochemical processes are involved in regulating the consecutive transition of different phases of dormancy in sweet cherry buds. An evaluation based on a metabolic approach has, as yet, only been partly addressed. The aim of this work, therefore, was to determine which plant metabolites could serve as biomarkers for the different transitions in sweet cherry buds. The focus here was on those metabolites involved in oxidation-reduction processes during bud dormancy, as determined by targeted and untargeted mass spectrometry-based methods. The metabolites addressed included phenolic compounds, ascorbate/dehydroascorbate, reducing sugars, carotenoids and chlorophylls. The results demonstrate that the content of phenolic compounds decrease until the end of endodormancy. After a long period of constancy until the end of ecodormancy, a final phase of further decrease followed up to the phenophase open cluster. The main phenolic compounds were caffeoylquinic acids, coumaroylquinic acids and catechins, as well as quercetin and kaempferol derivatives. The data also support the protective role of ascorbate and glutathione in the para- and endodormancy phases. Consistent trends in the content of reducing sugars can be elucidated for the different phenophases of dormancy, too. The untargeted approach with principle component analysis (PCA) clearly differentiates the different timings of dormancy giving further valuable information.
KW  - dormancy
KW  - redox-metabolites
KW  - phenolics
KW  - ascorbate
KW  - anti-oxidative capacity
KW  - Prunus avium L.
KW  - flower buds
Y1  - 2018
U6  - https://doi.org/10.3390/molecules23051197
SN  - 1420-3049
VL  - 23
IS  - 5
SP  - 1
EP  - 19
PB  - Molecular Diversity Preservation International
CY  - Basel
ER  - 
TY  - JOUR
A1  - Silva, Bibiana
A1  - Oliveira Costa, Ana Carolina
A1  - Tchewonpi, Sorel Sagu
A1  - Bönick, Josephine
A1  - Huschek, Gerd
A1  - Gonzaga, Luciano Valdemiro
A1  - Fett, Roseane
A1  - Baldermann, Susanne
A1  - Rawel, Harshadrai Manilal
T1  - Comparative quantification and differentiation of bracatinga (Mimosa scabrella Bentham) honeydew honey proteins using targeted peptide markers identified by high-resolution mass spectrometry
JF  - Food research international
N2  - Honey traceability is an important topic, especially for honeydew honeys, due to the increased incidence of adulteration. This study aimed to establish specific markers to quantify proteins in honey. A proteomics strategy to identify marker peptides from bracatinga honeydew honey was therefore developed. The proteomics approach was based on initial untargeted identification of honey proteins and peptides by LC-ESI-Triple-TOF-MS/MS, which identified the major royal jelly proteins (MRJP) presence. Afterwards, the peptides were selected by the in silico digestion. The marker peptides were quantified by the developed targeted LC-QqQ-MS/MS method, which provided good linearity and specificity, besides recoveries between 92 and 100% to quantify peptides from bracatinga honeydew honey. The uniqueness and high response in mass spectrometry were backed by further complementary protein analysis (SDS-PAGE). The selected marker peptides EALPHVPIFDR (MRJP 1), ILGANVK (MRJP 2), TFVTIER (MRJP 3), QNIDVVAR (MRJP 4), FINNDYNFNEVNFR (MRJP 5) and LLQPYPDWSWTK (MRJP 7), quantified by LC-QqQ-MS/MS, highlighted that the content of QNIDVVAR from MRJP 4 could be used to differentiate bracatinga honeydew honey from floral honeys (p < 0.05) as a potential marker for its authentication. Finally, principal components analysis highlighted the QNIDVVAR content as a good descriptor of the analyzed bracatinga honeydew honey samples.
KW  - Honeydew honey
KW  - Major royal jelly proteins
KW  - Marker peptides
KW  - High-resolution mass spectrometry
KW  - Principal component analysis
Y1  - 2020
U6  - https://doi.org/10.1016/j.foodres.2020.109991
SN  - 0963-9969
SN  - 1873-7145
VL  - 141
PB  - Elsevier
CY  - New York, NY [u.a.]
ER  - 
TY  - JOUR
A1  - Tchewonpi Sagu, Sorel
A1  - Landgräber, Eva
A1  - Henkel, Ina M.
A1  - Huschek, Gerd
A1  - Homann, Thomas
A1  - Bußler, Sara
A1  - Schlüter, Oliver
A1  - Rawel, Harshadrai Manilal
T1  - Effect of cereal α-amylase/trypsin inhibitors on developmental characteristics and abundance of digestive enzymes of mealworm larvae (Tenebrio molitor L.)
JF  - Insects : open access journal
N2  - The objective of this work was to investigate the potential effect of cereal α-amylase/trypsin inhibitors (ATIs) on growth parameters and selective digestive enzymes of Tenebrio molitor L. larvae. The approach consisted of feeding the larvae with wheat, sorghum and rice meals containing different levels and composition of α-amylase/trypsin inhibitors. The developmental and biochemical characteristics of the larvae were assessed over feeding periods of 5 h, 5 days and 10 days, and the relative abundance of α-amylase and selected proteases in larvae were determined using liquid chromatography tandem mass spectrometry. Overall, weight gains ranged from 21% to 42% after five days of feeding. The larval death rate significantly increased in all groups after 10 days of feeding (p < 0.05), whereas the pupation rate was about 25% among larvae fed with rice (Oryza sativa L.) and Siyazan/Esperya wheat meals, and only 8% and 14% among those fed with Damougari and S35 sorghum meals. As determined using the Lowry method, the protein contents of the sodium phosphate extracts ranged from 7.80 ± 0.09 to 9.42 ± 0.19 mg/mL and those of the ammonium bicarbonate/urea reached 19.78 ± 0.16 to 37.47 ± 1.38 mg/mL. The total protein contents of the larvae according to the Kjeldahl method ranged from 44.0 and 49.9 g/100 g. The relative abundance of α-amylase, CLIP domain-containing serine protease, modular serine protease zymogen and C1 family cathepsin significantly decreased in the larvae, whereas dipeptidylpeptidase I and chymotrypsin increased within the first hours after feeding (p < 0.05). Trypsin content was found to be constant independently of time or feed material. Finally, based on the results we obtained, it was difficult to substantively draw conclusions on the likely effects of meal ATI composition on larval developmental characteristics, but their effects on the digestive enzyme expression remain relevant.
KW  - growth behavior
KW  - Tenebrio molitor larvae
KW  - feeding
KW  - cereal meals
KW  - α-amylase
KW  - digestive enzymes quantification
KW  - LC-MS/MS
KW  - trypsin inhibitors
Y1  - 2021
U6  - https://doi.org/10.3390/insects12050454
SN  - 2075-4450
VL  - 12
IS  - 5
PB  - MDPI
CY  - Basel
ER  -