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Article
Impact of Conventional and Integrated Management Systems on the Water-Soluble Vitamin Content in Potatoes, Field Beans and Cereals Sabine Freitag, Susan R Verrall, Simon DA Pont, Diane McRae, Julia Anne Sungurtas, Raphaelle Palau, Cathy Hawes, Colin J Alexander, William J Allwood, Alexandre Foito, Derek Stewart, and Louise Shepherd J. Agric. Food Chem., Just Accepted Manuscript • DOI: 10.1021/acs.jafc.7b03509 • Publication Date (Web): 19 Dec 2017 Downloaded from http://pubs.acs.org on December 20, 2017
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Journal of Agricultural and Food Chemistry is published by the American Chemical Society. 1155 Sixteenth Street N.W., Washington, DC 20036 Published by American Chemical Society. Copyright © American Chemical Society. However, no copyright claim is made to original U.S. Government works, or works produced by employees of any Commonwealth realm Crown government in the course of their duties.
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Journal of Agricultural and Food Chemistry
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Impact of Conventional and Integrated Management Systems on the
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Water-Soluble Vitamin Content in Potatoes, Field Beans and
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Cereals
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Sabine Freitaga,*, Susan R. Verralla, Simon D.A. Ponta, Diane McRaea, Julia A. Sungurtasa,
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Raphaëlle Palaua, Cathy Hawesa, Colin J. Alexanderb, J. William Allwooda, Alexandre Foitoa,
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Derek Stewarta,c, Louise V.T. Shepherda
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a
Environmental and Biochemical Sciences, The James Hutton Institute, Invergowrie, Dundee
DD2 5DA, UK.
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b
Biomathematics and Statistics Scotland, Invergowrie, Dundee, DD2 5DA, UK.
13 14
c
15
UK.
School of Engineering and Physical Sciences, Heriot-Watt University, Edinburgh, EH14 4AS,
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*To whom correspondence should be addressed: Tel: + 44 (0)1382 568919; Email:
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[email protected] 1 ACS Paragon Plus Environment
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Abstract
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The reduction of the environmental footprint of crop production without compromising crop
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yield and their nutritional value is a key goal for improving the sustainability of agriculture. In
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2009, the Balruddery Farm Platform was established at The James Hutton Institute as a long-
31
term experimental platform for cross-disciplinary research of crops using two agricultural
32
ecosystems.
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integrated management systems, and analyzed for their water-soluble vitamin content.
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Integrated management, when compared with the conventional system, had only minor effects
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on water-soluble vitamin content, where significantly higher differences were seen for the
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conventional management practice on the levels of thiamine in field beans (p < 0.01), Spring
37
barley (p < 0.05) and Winter wheat (p < 0.05), and for nicotinic acid in Spring barley (p < 0.05).
38
However, for all crops, Variety and Year differences were of greater importance. These results
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indicate that the integrated management system described in this study does not significantly
40
affect the water-soluble vitamin content of the crops analyzed here.
Crops representative of UK agriculture were grown under conventional and
41 42 43 44 45 46 47 48 49
Key Words: barley (Hordeum vulgare L.), field beans (Vicia faba L.), integrated management,
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Liquid Chromatography-Triple Quadrupole-Mass Spectrometry, potato (Solanum tuberosum L.),
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water-soluble vitamins (WSVs), wheat (Triticum aestivum L.). 2 ACS Paragon Plus Environment
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Introduction
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UK1 and EU2 agricultural policies and strategies are geared towards a shift to a more sustainable
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use of resources and conservation of farmland biodiversity.
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understand the impact of the environment, crop management and soil fertility on both the yield
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and nutritional quality of economically important crops in Scotland. Currently, the long-term,
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systems-level impact of changes in management, especially in terms of sustainable treatment
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strategies, has been little studied.
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management whilst maintaining crop yield and nutritional quality. In 2009, The James Hutton
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Institute set up a long-term experimental platform3 for cross-disciplinary research on the use of
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both integrated and conventional management systems in agricultural ecosystems. The platform
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is based on a framework for designing and testing cropping systems that hopes to optimise the
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balance between crop yield and product quality on one hand, with biodiversity and ecosystem
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services on the other (in essence, attempting to assess the balance between economic and
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environmental demands). The aim is to reduce the environmental footprint of crop production
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by minimising the use of fossil fuel derived inputs and maximising the benefits from renewable
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resources. The long-term, whole-systems approach adopted at the platform is essential if the
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potential conflicts between food production and environmental health are to be reconciled. So
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far, much of the literature has focused on the effect of organic versus (vs.) conventional
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cultivation systems on nutritional value4-9, but also yield and cellular processes9-12 mainly in
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potatoes, whilst the impact of lower input (sustainable, organic, integrated) farming practices on
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crop nutritional value has rarely been investigated13,14. Conventional, integrated, sustainable and
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organic cultivation strategies have different goals in relation to crop yield, land and pesticide use,
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and also environmental impact. While conventional agricultural practices utilize high yield crop
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varieties, chemical fertilizers and pesticides, irrigation and mechanization, sustainable farming
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agricultural practices are designed to promote environmental health and the social and economic
Therefore, it is important to
There clearly is a need for balancing environmental
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equity of a region. Sustainable agriculture practices are hard to define as conditions can vary
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greatly depending on the crop, environment, and issues important to a region13.
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The term “nutritional value” as such has been defined as the chemical composition of food, in
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particular the amounts of key compounds that are essential for functioning of human
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organisms15. Vitamins are a broad group of organic bioactive compounds that are minor but
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nutritionally-essential constituents of food. Generally, vitamins can be divided into fat soluble
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(vitamin A, D, E and K1) and water-soluble vitamins (WSVs), which include the B-group
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vitamins thiamine (B1), riboflavin (B2), pyridoxine (B6), nicotinic acid (B3), pantothenic acid
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(B5) and vitamin C. These act as coenzymes, and are therefore essential for a range of different
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metabolic processes16. Most vitamins, apart from vitamin D and nicotinic acid, are essential in
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the human diet as the body cannot synthesize them. With the exception of vitamin B12, only
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plants have the ability to synthesize B vitamins17. Post-harvest processing (such as drying,
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storage, dehulling, milling, soaking, blanching, fermentation and cooking) can impact the levels
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of WSVs in various crops18,19, however, the number of studies on the effects of pre-harvest
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conditions (particularly different agricultural management practices) on content of WSVs have
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been limited. Most studies in the literature, on the impact of different cropping systems on WSV
95
contents, have focused on vitamin C content in some fruits, vegetables and eggs8,20-24. Whilst
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vitamin C is generally the most studied vitamin, little data have been published on other B
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vitamin levels in food crops.
98 99
The major challenge previously in quantifying WSVs has been sensitivity, as the low levels in
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crops (such as cereals) require very sensitive methods25, and their simultaneous quantification of
101
these diversely different chemistries.
102
quantification of single vitamins, e.g. Martins-Junior et al.26, and methods range from
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microbiological assays17, Biosensor/ELISA27 to chromatographic procedures with UV or
Previous methods have mainly focused on the
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fluorescence detection28,29. These extraction and detection methods have several drawbacks
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including the number of B vitamins quantified, lack of precision and their sensitivity. Only
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recently have advances been made regarding increased sensitivity and simultaneous detection of
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WSVs in various food matrices ranging from maize flour, tomato pulp, kiwi to semi-coarse
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wheat flour, wheat bread and toasted wheat bread30,31. Liquid chromatography-triple quadrupole
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mass spectrometry has been optimized as a rapid procedure for multivitamin quantification in
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combination with an optimized extraction procedure30,31. For this study, a method by Nurit et
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al.31 has been adapted to investigate whether our integrated management system impacts upon
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the content of five WSVs in a range of different crop matrices - including field beans (Vicia faba
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L.), Spring and Winter barley (Hordeum vulgare L.), Winter wheat (Triticum aestivum L.) and
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potato (Solanum tuberosum L.) – the latter of which was also analyzed for vitamin C content.
115 116
Material and Methods
117 118
Experimental Design and Preparation of Sample Material
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The Balruddery Farm platform, Dundee3 comprises a 42 hectare (ha) contiguous block of six
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arable fields, north-east Scotland (56.48 latitude-3.13 longitude). Balruddery Farm is a 178 ha
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arable farm, 67 to 163 m above sea level on the south facing slopes of the Sidlaw Hills. The
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farm is typical of temperate Atlantic maritime arable environments, with an average annual
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rainfall of 800 mm, an average annual accumulated temperature of 1100-1375 day oC (above 5.6
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o
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(2.6-4.4 metres second-1 wind speed) and has moderate winters of 50-110 day oC of accumulated
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frost. The soils are imperfectly draining Balrownie Series32 with an average pH of 5.7. Topsoil
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depths range from 25-40 cm, textures from sandy loam to sandy silt loam and stone contents of
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10-20 % volume. Each of the six fields are divided in half, and the integrated and conventional
C) and a mean annual potential water deficit of 50-75 mm. The area is moderately exposed
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management systems randomly allocated to each field half in 2010, at the start of the first
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rotation (Figure 1)3. These systems then remain in place for the duration of the experiment to
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allow detection of a build-up in response to cropping system over time.
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management system is a composite treatment, including tram-line management in cereals and
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tied-ridging in potatoes to reduce soil, water and nutrient loss33; non-inversion tillage to improve
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physical structure and decrease nutrient losses34; green waste compost addition and crop residue
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incorporation to build-up soil carbon and improve physical structure35; green cover (forage
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radish) over Winter before potato to reduce nitrogen (N) losses and increase phosphorous (P)
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uptake36; clover under sowing of Spring barley crops for additional renewable N input to the
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rotation37; lower doses of artificial N fertilizer (taking approximately 75 % of the standard rate as
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a reasonable starting point for this site, based on expert agronomic advice, with further
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reductions planned as soil fertility improves) to reduce environmental footprint, leaching and
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emissions38; lower herbicide dose and alternative chemicals to encourage a diverse weed
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understorey, aiming at approximately 10 % ground cover of non-competitive dicotyledonous
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weeds39, and threshold crop protection applications based on the Home-Grown Cereals Authority
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(HGCA), now the Agriculture and Horticulture Development Board (AHDB) dose response
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curves40 (Table 2). The crop rotation is potato followed by Winter wheat, Winter oilseed rape,
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Winter barley, field (Spring) beans and Spring barley. These crops were selected as typical for
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the Tayside farming region and representative of the most common cropping systems in Scotland
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(and much of the UK). Winter crops are sown in late summer/autumn (August-October) and
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harvested the following summer (July-September). Spring crops are sown between March and
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May, and harvested August-September of the same year. Within each half-field, five different
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varieties of each crop were sown to assess variety-specific responses to the change in
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management systems. For each crop, one variety was selected which was an industry standard,
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providing a comparator to annual UK performance. The remaining varieties were selected for
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specific environmental traits such as disease resistance, resource use efficiency and weed
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tolerance3 (Table 1). Table 1. Summary of crops, and their varieties, used for the analysis of water-soluble vitamins over five years.
Crop
Potato
Field Beans
Spring Barley
Winter Barley
Winter Wheat
Year 1
Year 2
Year 3
Year 4
Year 5
2010/2011
2011/2012
2012/2013
2013/2014
2014/2015
Cabaret
Cabaret
Cabaret
Cabaret
Cabaret
Lady Balfour
Lady Balfour
Lady Balfour
Lady Balfour
Lady Balfour
Maris Piper
Maris Piper
Maris Piper
Maris Piper
Maris Piper 1
Mayan Gold
Mayan Gold
Mayan Gold
Mayan Gold
Maris Piper 2
Vales Sovereign
Vales Sovereign
Vales Sovereign
Vales Sovereign
Vales Sovereign
Ben
Ben
Ben
Babylon
Babylon
Fuego
Fuego
Fuego 1
Boxer
Boxer
Maris Bead
Maris Bead
Fuego 2
Fanfare
Fanfare
Pyramid
Pyramid
Pyramid
Fuego
Fuego
Tattoo
Tattoo
Tattoo
Pyramid
Pyramid
4-Component Mix
4-Component Mix
4-Component Mix
4-Component Mix
4-Component Mix
Concerto
Concerto
Concerto
Concerto
Concerto
Optic
Optic
Optic
Optic
Optic
Waggon
Waggon
Waggon
Waggon
Waggon
Westminster
Westminster
Westminster
Westminster
Westminster
4-Component Mix
4-Component Mix
4-Component Mix
4-Component Mix
4-Component Mix
Flaggon
Cassata
Cassata
Cassata
Cassata
Retriever
Retriever
Retriever
Retriever
Retriever
Saffron
Saffron
Saffron
Saffron
Saffron
Sequel
Sequel
Sequel
Sequel
Sequel
Alchemy
Alchemy
Alchemy
Alchemy
Alchemy
Consort
Beluga
Beluga
Beluga
Beluga
Istabraq
Consort
Consort
Consort
Consort
Viscount
Istabraq
Istabraq
Istabraq
Istabraq
Zebedee
Viscount
Viscount
Viscount
Viscount
Where Bold text denotes the industry standard.
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For Spring barley, the same four varieties, and a four-component mix (4-Comp Mix), comprising
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each of those varieties, were grown over 2011-2015. However, for the other crops, adjustments 7 ACS Paragon Plus Environment
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had to be made as to which varieties were grown in each year, depending on seed availability.
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For example, the potato variety Mayan Gold was not available for growth in 2015, however, no
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alternative variety was substituted, rather Maris Piper (the industry standard) was grown in two
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adjacent plot strips (Table 1). For Winter wheat in 2011, Beluga was not available, and Zebedee
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was grown in its place. Similarly, for Winter barley in 2011, Cassata was not available and
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Flaggon was grown in its place. This had implications for the 4-Comp Mix in 2011, as it was not
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comparable with the 4-Comp Mixes generated for Winter barley in 2012-2015. Field beans were
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more complex, where only two varieties – Fuego and Pyramid, were consistently grown over
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2011-2015. Two of the varieties – Ben and Tattoo were only grown over 2011-2013. Maris
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Bead was only grown over 2011-2012. Finally, Babylon, Boxer and Fanfare were available for
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2014-2015. This meant that in total, over the five years, eight varieties of field beans were
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grown. The above has been considered, and factored into the resulting statistical outputs, which
171
will be explained in the Statistical Analysis section.
172 173
Cereals and potatoes were harvested from 1 m x 1 m quadrats at five, fixed Global Positioning
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System (GPS) locations in each variety strip as indicated in Figure 1. With regards to the field
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beans, the GPS locations were not physically accessible in the standing crop without causing pod
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shatter and yield loss. Therefore, after each variety strip was harvested, five hand-sampled
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aliquots were collected (providing five technical, rather than spatial, replicates) for WSV
178
analysis.
179 180
Following harvest, the sample material was prepared as follows: the three cereal crops were
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dried down to industrial standards (10-15 % moisture still present), threshed with a small
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combine harvester, and then graded (barley: sieve size of 2.5 mm; wheat: sieve size of 2.25 mm).
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The seeds were then milled with Retch ZM 200 ultra-centrifugal mill (Tecator Udy, sieve size
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0.5 mm). The milled powders were then individually packed in polyethylene bags (VWR, UK)
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and stored at -20 °C until required for analysis.
186 187
After the potato harvest, the potato tubers were stored in the dark at ambient temperature for a
188
minimum of one week to facilitate skin set - the common UK post-harvest practice. For each
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replicate (GPS point), four to five average-sized potato tubers, with a combined fresh weight of
190
approximately 800 g, were selected, washed by hand, and each tuber then transected into eight
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segments. Two diametrically opposed segments (taken to provide a representative sample of the
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whole tuber) were taken from each tuber, and the opposite eighths from the tubers per replicate
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combined, then flash frozen in liquid N and stored at -20 °C. The frozen material was then
194
freeze-dried for five days, then the dried material milled using a Retch ZM 200 ultra-centrifugal
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mill (Tecator Udy; 0.5 mm sieve). The milled potato powders were then individually packed in
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polyethylene bags (VWR, UK) and stored at -20 °C (in the dark) until required for analysis.
197 198
Five ‘replicate’ aliquots of field beans, each comprising 60 beans, were flash frozen in liquid N,
199
stored at -20 °C, freeze dried overnight, then milled as per the potatoes. The milled field bean
200
powders were then individually packed, as for potato, and stored at -20 °C (in the dark) until
201
required for analysis.
202 203
Chemicals and Reagents
204 205
All chemicals used for the present study were of analytical grade (purity > 98 %). Analytical
206
standards of thiamine hydrochloride, nicotinic acid, pyridoxine hydrochloride, pantothenic acid,
207
and riboflavin were obtained from Scientific Laboratory Supplies Ltd (Newhouse, UK).
208
Individual stock solutions for all five vitamins were prepared in 50:50 (v/v) acetonitrile/water (4
209
mg mL-1). A stock solution of all five vitamins was prepared in 50:50 (v/v) acetonitrile/water 9 ACS Paragon Plus Environment
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with a concentration of 100 µg mL-1. The labelled internal standard pantothenic acid-13C3,15N
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hemicalcium salt was obtained from LGC Standards (Teddington, UK). Thiamine-4-methyl-13C-
212
thiazol-5-yl-13C hydrochloride and pyridoxal-methyl-d3 were purchased from Sigma Aldrich
213
(Dorset, UK). Internal standard solutions were prepared by dissolving 1 mg in 1 mL 50:50 (v/v)
214
acetonitrile/water. Prior to batch extraction, a mix of all three internal standard solutions was
215
prepared resulting in a final concentration of 13.6 mg mL-1. Sodium acetate trihydrate, glyoxylic
216
acid monohydrate, L-glutathione reduced, ethylenediaminetetraacetic acid (EDTA), sodium
217
hydroxide, iron(II) sulphate heptahydrate, formic acid and glacial acetic acid were purchased
218
from Fisher Scientific (UK, Analytical Grade). Tris(2-carboxyethyl)phosphine hydrochloride
219
(TCEP), metaphosphoric, sulphuric and ascorbic (AsA) acids were purchased from Sigma
220
Aldrich (Dorset, UK). HPLC grade acetonitrile was purchased from VWR (West Sussex, UK).
221
Ultrapure water (18.2 MΩ.cm) was obtained from an Elga Purelab-Option Q System (High
222
Wycombe, UK).
223 224
Quantification of Vitamin C
225 226
The vitamin C content of freeze-dried potato powders were quantified as follows: 100 mg of
227
powder was weighted into 2 mL microfuge tubes and resuspended in 1 mL of 5 % (w/v)
228
metaphosphoric acid containing 5 mM TCEP, which acts as a reducing agent by converting
229
dehydroascorbate (DHA) to AsA. Consequently, results are presented as total vitamin C (total
230
AsA). The suspension was vortexed for 10 seconds and transferred onto a blood rotator for 30
231
min at 5 °C. Following this, the suspension was centrifuged at 5 °C for 10 min. The supernatant
232
was then transferred into a clean 2 mL microfuge tube, and the remaining pellet re-extracted as
233
before. Both extracted supernatants were combined, centrifuged to pellet any remaining debris,
234
and the supernatant transferred into 0.3 mL transparent polypropylene-short threaded High-
235
Performance Liquid Chromatography (HPLC) micro-vials sealed with a 9 mm polypropylene 10 ACS Paragon Plus Environment
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screw cap (VWR, UK), and subjected to HPLC (ASI-100 autosampler, and Ultimate 3000 pump)
237
coupled to a UV-Visible detector (UVD340U, Dionex, ThermoFisher SCIENTIFIC, UK).
238
Autosampler and column temperature were maintained at 4 °C and 50 °C respectively. 20 µL of
239
sample was injected onto an ICSep COREGAL-64H column (ChromTech, USA), with the
240
dimensions of 7.8 x 300 mm and particle size of 10 µm and cross linkage of 6.4. An isocratic
241
run of 30 min was applied with a mobile phase containing 4 mM sulphuric acid in ultrapure
242
water. AsA was detected by absorbance using a diode array detector and quantified at 245 nm.
243
Quantification was performed at 245 nm against external calibration of AsA in a range of 20-75
244
µg mL-1.
245 246
Sample Extraction, Dilution and Preparation of the Standard Curve for Quantification of
247
WSVs
248 249
Extraction procedures followed the protocol from Nurit et al.31 and were as follows: for
250
extraction 622 mg (± 2 mg) were weighted into 50 mL tubes (Sarstedt, Germany). Following
251
this, 100 µL of internal standard solution (13.6 µg mL-1) was added in addition to 4.75 mL of
252
sodium acetate (pH 4.5, concentration of 0.5 mM, pH adjusted with glacial acetic acid), 1.25 mL
253
of 0.5 M glyoxylic acid solution, 0.25 mL of 1 % (v/v) L-glutathione reduced solution, 0.25 mL
254
of 1 % ethylene-diamine-tetraacetic acid solution (adjusted with NaOH for solubility) and 0.2
255
mL of 2 % iron(II) sulphate heptahydrate to the powder. The mixture was strongly mixed for 30
256
seconds using a vortex, and then incubated in the dark at 37 °C for 16 h on a shaker (1,500 rpm).
257
Following this, the cooled sample was vortexed and centrifuged at 12,000 g for 10 min at 3 °C.
258
The supernatant was filtered through a 0.22 µm filter vial (Polytetrafluoroethylene; PTFE) with a
259
pre-slit cap (Thomson, BioProcess Engineering Services Ltd, Kent, UK).
260
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Reference materials were prepared to account for extraction, but also instrument stability (see
262
Supporting Information; Reference Generation and Quality Control, and Tables S2-S6).
263 264
Chemical Analysis
265 266
Chemical analysis of the potato, field bean and cereal powders were performed on an Agilent
267
1260 HPLC system consisting of a quaternary pump, a Diode Array Detector (DAD), a
268
Temperature Control Device, and a solvent Thermostat module (Agilent Infinity 1290) coupled
269
to an Agilent 6460A Triple Quadrupole Mass Spectrometer (Agilent Technologies, Santa Clara,
270
CA, USA). Sample extract (5 µL) was injected onto a 100 x 3 mm (2.5 µm) Synergy Hydro-RP
271
C18 column with polar end capping, fitted with an AQ C18 4 x 2 mm security guard TM
272
cartridge (Phenomenex, Cheshire, UK). Samples were eluted at a flow rate of 0.5 mL min-1
273
using a gradient consisting of two mobile phases: A = 0.1 % (v/v) formic acid in deionized water
274
and B = 100 % acetonitrile. The elution gradient was as follows: A/B 98/2 (v/v) hold for 2 min;
275
ramped up from 2 to 60 % B in 3 min and hold for 1 min, and further ramped up from 60 % to 90
276
% in 0.1 min and hold for 1.9 min. Within 0.1 min the gradient was returned to the initial
277
composition and held for 5 min until the next injection. One analytical run lasted 13.1 min
278
(Supplementary Information, Figure S2).
279 280
Mass detection was carried out in positive ion mode for all vitamins apart from the isotopically
281
labelled pantothenic acid (pantothenic acid
282
(ESI) interface coupled to the triple quadrupole system. For ESI, the gas temperature, gas flow,
283
nebulizer pressure, sheath gas temperature, sheath gas flow, capillary cap voltage and nozzle
284
voltage were set to 350 °C, 11 L min-1, 50 psi, 300 °C, 11 L min-1, 4 kV (3 kV for negative ion
285
mode) and 500 V, respectively. Collision energies for transition states of the five standard
286
compounds including thiamine, nicotinic acid, pyridoxine, pantothenic acid and riboflavin, as
13
C3,
15
N) using a jet stream electrospray ionisation
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well as the isotopically labelled internal standards thiamine-4-methyl-13C-thiazol-5yl13C,
288
pyridoxal methyl-d3, pantothenic acid 13C3, 15N, were optimized for optimal fragmentor voltage
289
and collision energies (Supporting [S] Information, Table S1).
290
transitions, i.e. transitions with the highest intensity of the product ions were chosen to build the
291
final multiple reactions monitoring (MRM) method. As shown in Table S1, 16 transitions were
292
part of the MRM mode, each with a dwell time of 20 milliseconds (ms) and a delay time of 3.5
293
ms, leading to a total cycle time of 376 ms, and thus 2.7 cycles per second. Peaks of the five B
294
vitamins and three labelled B vitamins were integrated with Agilent MassHunter Quantitative
295
Software (Agilent, USA).
Hereby, the most sensitive
296 297
Quantification of the WSVs
298 299
As listed in Table S1, seven protonated molecular ions [M+H]+ and one deprotonated molecular
300
ion [M-H]- (pantothenic acid-13C3,15N) were chosen as precursor ions in the MS/MS (tandem
301
Mass Spectrometry) experiment. For confirmation, qualifier ions were also included in the
302
method. The most abundant product ions were used for quantification, measured in MRM mode.
303
A ten-point calibration curve for each B vitamin in the potato, field bean and cereal samples
304
were calculated ranging from 2 ng mL-1 up to 1 µg mL-1. As in Nurit et al.31, calibration curve
305
standards were prepared by adding 100 µL of mix unlabelled external standards (10 ng mL-1–5
306
µL min-1) into microfuge tubes containing 100 µL of thiamine-4-methyl-13C-thiazol-5-yl-13C
307
hydrochloride (1 µL min-1), 100 µL pantothenic acid-13C3,15N hemicalcium salt (1 µL min-1),
308
100 µL pyridoxal-methyl-d3 (1 µL min-1) and 100 µL of acetonitrile/water (50:50; v/v). Due to
309
matrix effects, the response ratio of each vitamin was calculated against a labelled internal
310
standard of the same or as similar chemistry as possible: thiamine with thiamine-4-methyl-13C-
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thiazol-5-yl-13C hydrochloride; riboflavin and pantothenic acid with pantothenic acid-13C3,15N
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hemicalcium salt and pyridoxine and nicotinic acid with pyridoxal-methyl-d3. 13 ACS Paragon Plus Environment
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Statistical Analysis
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A separate statistical analysis was performed on the vitamin measurements for each crop using a
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linear mixed model approach. The two main effects of Variety and Input (management system)
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were fitted as fixed effects along with an interaction term. In addition, the effect of Year was
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analyzed as a fixed, rather than random, effect since variance component estimates with so few
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levels can be unreliable. The Years here are considered as experimental replicates and account
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for variability in field and environmental conditions. Three of the terms in the random model
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account for the physical layout of the design. The nested block terms of Replicate (Rep; samples
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taken at the five GPS points, except for field beans, as described below) within Variety strip
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within half-field were fitted as random effects. In addition, interaction terms for Year×Variety,
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Year×Rep and Year×Input×Rep were also included as random effects. The Year×Variety term
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has been found to be a particularly important component of variance, and necessary for a good
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model fit. The terms for Year×Rep and Year×Input×Rep capture further sources of variance
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within the field. They also account for any variation due to the order in which samples were
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processed in the laboratory stage, as during an analysis run Rep blocks are processed in a
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sequence with sample order randomised within these (see Supporting Information).
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Between years there were changes to the selection of varieties grown for field beans, Winter
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wheat, Winter oilseed rape and Winter barley (Table 1). Varieties which were present in only
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one year (Winter wheat – variety Zebedee and Winter barley – variety Flaggon) were excluded
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from the analysis.
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Data from field beans had a slightly different structure in that the five samples from each strip
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were technical replicates, rather than spatial.
However, the same model was used since
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Year×Rep and Year×Input×Rep terms were still required to capture variability in laboratory
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processing of the technical Rep blocks.
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The complexity of the experimental design meant that there were many potential random effects
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which were difficult to estimate in combination. The model we selected here ensured that the
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fixed effects were estimated against the appropriate level of random variation with degrees of
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freedom estimated from the design. Measured values were logarithmically transformed to base
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10 (log10) before the analyses to account for variance heterogeneity in the residuals. All analyses
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were performed using Restricted Maximum Likelihood (REML) procedures in GenStat for
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Windows 17th edition (VSN International Ltd., Hemel Hempstead, UK).
349 350
Results
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Five WSVs (nicotinic acid, pyridoxine, thiamine, riboflavin and pantothenic acid; Figure S1)
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were quantified in five varieties of five different crops - potato, Spring barley, Winter barley,
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Winter wheat and field beans. For potato, vitamin C content was also quantified due to its intake
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being of high importance in western diets41,42.
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In potato, highly significant differences (p < 0.001; thiamine p < 0.01; Table 3) in all six vitamin
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concentrations were seen in all five varieties (Table S8). Most obvious from Table S8 were the
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levels of nicotinic acid, which varied from ~1 – 46 µg g-1 DW, between the varieties (p < 0.001).
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Cabaret had the lowest nicotinic acid levels, whereas the levels in Vales Sovereign were 7-40-
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fold higher when compared with the other four varieties. Cabaret also had the lowest levels of
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pantothenic acid, riboflavin and thiamine concentrations when compared with the other four
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varieties. Broadly speaking, Vales Sovereign had the highest concentrations of pantothenic acid,
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pyridoxine and vitamin C. Figure 2 shows that Input did not significantly (Table 3) affect the
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concentrations (Table S8) of any of the six vitamins quantified over the five years studied.
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Table 3 (and Table S9) show significant differences were observed across the field beans
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varieties in the concentrations of nicotinic acid (p < 0.05), pyridoxine (p < 0.01) and riboflavin
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(p < 0.001). Figure 3 (and Table S9) shows that the variety Ben had the lowest levels of
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nicotinic acid compared to the other seven varieties - Maris Bead, Boxer, Fanfare, Fuego,
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Babylon, Pyramid, and Tattoo. The lowest concentration of pyridoxine was found in Maris
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Bead, whereas this variety had the highest concentrations of riboflavin. With the exception of
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thiamine (Figure 3), whose concentration was significantly lower (p < 0.01) in varieties grown
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under the integrated management system (Table 3), Input did not significantly affect any of the
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other analyzed vitamins (Table S9).
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For Spring barley, with the exception of thiamine (Table S10), highly significant variety
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differences (p < 0.001; Table 3) were observed in the concentrations of four of the WSVs
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analyzed. As observed for the field beans, Input only affected the concentration of thiamine
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(Figure 4), which again was lower (p < 0.05; Table 3) in varieties grown under the integrated
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management system (Table S10).
382 383
Table 3 shows that for Winter barley all five WSV concentrations had highly significant (p