Effect of Orchard Management Factors on Flesh Color of Two Red-Fleshed Apple Clones


horticulturae

Article

Effect of Orchard Management Factors on Flesh Color
of Two Red-Fleshed Apple Clones

Annika Wellner, Eckhard Grimm * and Moritz Knoche

Institute for Horticultural Production Systems, Leibniz-University Hannover, Herrenhäuser Straße 2,
30419 Hannover, Germany
* Correspondence: eckhard.grimm@obst.uni-hannover.de; Tel.: +49-511-762-8081

Received: 23 May 2019; Accepted: 23 July 2019; Published: 29 July 2019
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Abstract: Little is known about factors affecting anthocyanin biosynthesis in red-fleshed apples
(Malus × domestica Borkh.). The objective was to establish the effects of orchard management factors
on flesh anthocyanin content of dark-colored (DC) and light-colored (LC) apple clones. Flesh color
was assessed by measuring color in the L, a, b mode using a spectrophotometer and predicting the
anthocyanin content based on relationships between the absorption of a flesh extract at 530 nm and
the L-value determined using a spectrophotometer (r2 = 0.99 ***). Fruit from the DC clone were red
by 86 days after full bloom (DAFB), whereas the LC clone began to color at 136 DAFB. Color intensity
in both clones decreased from the top of the tree to the base. Further, the intensity of the flesh color of
the DC clone decreased with shading (94% absorption of incident photosynthetic active radiation).
Covering a fruit with a UV absorbing film (100% UV absorption) had no effect on flesh color in the
DC clone but decreased color in the LC clone. Fruit thinning increased color in DC and LC fruit.
There was little change in flesh color during storage. However, the DC clone developed severe flesh
browning as storage progressed beyond 30 days. The results demonstrated that light (visible and
UV wavelength) stimulated, whereas shade inhibited, anthocyanin biosynthesis in the flesh under
orchard conditions.

Keywords: Malus × domestica; anthocyanin; canopy; light interception; parenchyma; crop load;
UV light

1. Introduction

The red blush of apple fruit skin is an important quality attribute. Recently, some apple genotypes
have become available that also have red-flesh. In these genotypes, the red color in the skin extends into
the flesh of the fruit. Red-fleshed apples are novel, and this makes them attractive to consumers and so
of increased economic value. A number of red-fleshed apple genotypes have now been identified and
evaluated [1–3]. Red fleshed genotypes fall into two categories, types 1 and 2. Type 1 genotypes are
strongly pigmented and dark-colored. The flesh color forms early during fruit development and the
leaves and shoots are also colored. In type 1 genotypes, the transcription factor MdMYB10 is involved
in regulating the biosynthesis of anthocyanins. Type 2 genotypes are less color intensive. Coloration
begins late in development, and leaves and shoots are without red color. In type 2 genotypes the
transcription factor MdMYB110a is involved in the regulation of biosynthesis of anthocyanin [4–6].

The pigments responsible for the red flesh are anthocyanins. In general, these may appear in
stems, leaves, flowers or fruits. The principle function of coloration is to make a plant or a plant organ
attractive to animals which act as vectors, carrying pollen and dispersing seeds. High anthocyanin
concentrations in fruit and vegetables are also considered beneficial in the human diet because of their
antioxidant [7], anticancer and antiaging properties [8,9].

Horticulturae 2019, 5, 0054; doi:10.3390/horticulturae5030054 www.mdpi.com/journal/horticulturae

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Horticulturae 2019, 5, 0054 2 of 11

The concentration of anthocyanin in the flesh and hence color intensity depends not only on
the genotype but also on environmental variables. For example, the anthocyanin content of a type
1 genotype varied by 14% depending on the site of production [10]. In addition, both light and
temperature affected anthocyanin biosynthesis in apple, and hence the skin and flesh color; for review
see [11,12]. Little is known about the effect of orchard management factors during cultivation on color
development in apple flesh.

The objective of our study was to establish the effects of orchard management factors on
anthocyanin content of a dark-colored (DC, type 1) and a light-colored (LC, type 2) apple clone.
We focused on factors related to light exposure because light affects anthocyanin biosynthesis in
the skin and may, therefore, also play a role in the flesh. The two apple clones examined here are
representative of the small range of DC and LC type apple fruits currently available.

2. Materials and Methods

2.1. Plant Material

Two red-flesh apple (Malus × domestica Borkh.) clones were selected that had dark-red (DC) and
light-red (LC) flesh (IFORED SAS, Seiches-sur-le-Loire, France). Trees were grafted on M9 rootstocks
and grown at the Obstbauzentrum Jork, Jork, Germany (53.5 N, 9.7 E) according to current practices of
integrated fruit production. Fruits were harvested during the season beginning at 86 days after full
bloom (DAFB) and were processed immediately or stored at 2 ± 1 ◦C pending analysis.

2.2. Quantifying Redness of Cross-Sections

For rapid quantification of the redness of the flesh, a procedure based on image analysis of digital
photographs was established. Flesh slices (3–5 mm thick) were excised from the equatorial plane of DC
and LC fruits. Equatorial slices were photographed using a Canon EOS 550 D camera equipped with
Macro lens EF-S 18–55 mm (Canon, Tokyo, Japan) mounted on a photo stand (RB 5000 DL, No. 5556 +
Prolite 5000, No. 2190; Kaiser Phototechnik, Buchen, Germany) equipped with three fluorescent tubes
(Osram TC-L, code 954, 5400 K), two above (36 W each) and one (15 W) in a lightbox underneath the
specimen. Images were taken together with the RHS color standards (Charts No. 39, 43, 45, 46; Royal
Horticultural Society, London, UK) and the ColorChecker (X-Rite Pantone; Grand Rapids, MI, USA)
as shown in Figure 1a. Images were processed using image analysis software (cellSens Dimension
1.7.1; Olympus, Hamburg, Germany) and the following procedure. First, the white standard was
calibrated. Second, the cross-section of the flesh was partitioned into four zones of different color
intensity. The limits for the different intensities were set according to the RHS color charts (No. 39,
43, 45, 46), as shown by false colors in Figure 1b. As for any one of the color charts the L-, a- and
b-coordinates were pre-determined (CM-2600d; Konica Minolta, Osaka, Japan) [13], a mean L-, a mean
a- or a mean b-value could be calculated that were weighted by the respective area of the cross-section.



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Figure 1. (a) Image of the equatorial slice of a red-fleshed apple that was taken together with four red 
color charts (No. 39, 43, 45, 46) of the Royal Horticultural Society (RHS) and a grey scale of 
ColorChecker. Red color charts and grey scale served as calibration. (b) False-color image of the 
photograph depicted in A. The four color classes were identified based on the L-values of the RHS 
color charts. 

2.3. Experiments 

A developmental time course was established by sampling the DC clone from 86 DAFB and the 
LC clone from 96 DAFB to maturity. 

Flesh color was recorded as a function of the position of the fruit in the canopy and the 
exposure of the fruit relative to the sun. The three positions in the canopy were: in the upper third of 
the crown (‘top’), in the middle third (‘middle’) and in the lower third (‘bottom’). Exposure relative 
to the sun was also varied by selecting fruit from the north- or south-exposed flanks of the row.  

Flesh color was recorded as a function of shading. Shading was achieved by wrapping 
individual branches in the middle of the tree with a hail net. Branches without net served as control. 
The light intensity in the shade treatment was only about 6% (LI-COR 
Quantum/Radiometer/Photometer LI250; Heinz Walz GmbH Mess- und Regelungstechnik, 
Effeltrich, Germany).  

Flesh color was recorded as a function of UV exposure. Fruits in the middle of the crown were 
covered with a UV-absorbing film (UV Schutzfolie Klar UV 3 SR; Özek and Wagner, Cologne, 
Germany). This film blocked all UV radiation as determined using a UV meter (sensor: type 2.5; 
Indium Sensor GmbH, Neuenhagen, Germany; data logger: Almemo® 2590-4AS; Ahlborn Mess- und 
Regelungstechnik GmbH, Holzkirchen, Germany). Fruit in the same position but without film 
served as control.  

Flesh color was recorded as a function of three levels of fruit thinning: no thinning, medium 
thinning and heavy thinning. Thinning was done by hand after terminal bud set. The mean number 
of fruits was 200, 120 and 50 per DC and 120, 80 and 30 per LC tree for the light, medium and heavy 
thinning treatments, respectively. The mean trunk cross-sectional area (0.6 m above graft union) was 
13.37 cm2 and 13.74 cm2 for DC and LC trees, respectively.  

The effect of storage duration on flesh color was quantified during 98 d of cold storage at 4 °C.  

2.4. Data Analysis 

All experiments were carried out with a minimum of 20 fruit sampled from a minimum of four 
trees. Unless individual fruit data are shown, data are means ± standard errors. Where error bars are 
not shown, they were smaller than the plotted symbols. Data were analyzed by analysis of variance 
(Proc GLM) and regression analysis (Proc REG) using the statistical software package SAS (version 
9.1.3; SAS Institute, Cary, NC, USA). Means were compared using Tukey’s Studentized Range 
(HSD) Test. The significances of coefficients of determination (r²) at P ≤ 0.001 are indicated by ***. 
  

Figure 1. (a) Image of the equatorial slice of a red-fleshed apple that was taken together with four
red color charts (No. 39, 43, 45, 46) of the Royal Horticultural Society (RHS) and a grey scale of
ColorChecker. Red color charts and grey scale served as calibration. (b) False-color image of the
photograph depicted in A. The four color classes were identified based on the L-values of the RHS
color charts.

To relate the L-, a- and b-values determined on cross-sections of the fruit to the anthocyanin
content of the tissue, a calibration curve was established. Briefly, tissue cylinders (12 mm diameter ×
3–5 mm long) were excised from the equatorial plane of DC and LC fruits. Cylinders were selected for
homogeneity of color ranging from white to dark red. The color of cylinders was quantified using
a spectrophotometer (CM-26001; Konica Minolta). Thereafter, cylinders were extracted using 1%
HCl in methanol (8 mL per cylinder) at room temperature overnight (>12 h). The absorption of the
extract was quantified spectrophotometrically at 530 nm (Specord 210; Analytik Jena, Jena, Germany).
An exponential regression model was fitted between absorption of the extract at 530 nm and the L-
and the a-value. Statistical analysis revealed highly-significant relationships between the absorption at
530 nm and the L- or the a-value determined on the same tissue cylinder. The regression equation
allowed conversion of any L-value (or a-value) of the three-dimensional color space determined on a
fruit cross-section, to an anthocyanin absorption value determined on a flesh extract.

2.3. Experiments

A developmental time course was established by sampling the DC clone from 86 DAFB and the
LC clone from 96 DAFB to maturity.

Flesh color was recorded as a function of the position of the fruit in the canopy and the exposure
of the fruit relative to the sun. The three positions in the canopy were: in the upper third of the crown
(‘top’), in the middle third (‘middle’) and in the lower third (‘bottom’). Exposure relative to the sun
was also varied by selecting fruit from the north- or south-exposed flanks of the row.

Flesh color was recorded as a function of shading. Shading was achieved by wrapping individual
branches in the middle of the tree with a hail net. Branches without net served as control. The light
intensity in the shade treatment was only about 6% (LI-COR Quantum/Radiometer/Photometer LI250;
Heinz Walz GmbH Mess- und Regelungstechnik, Effeltrich, Germany).

Flesh color was recorded as a function of UV exposure. Fruits in the middle of the crown were
covered with a UV-absorbing film (UV Schutzfolie Klar UV 3 SR; Özek and Wagner, Cologne, Germany).
This film blocked all UV radiation as determined using a UV meter (sensor: type 2.5; Indium Sensor
GmbH, Neuenhagen, Germany; data logger: Almemo® 2590-4AS; Ahlborn Mess- und Regelungstechnik
GmbH, Holzkirchen, Germany). Fruit in the same position but without film served as control.

Flesh color was recorded as a function of three levels of fruit thinning: no thinning, medium
thinning and heavy thinning. Thinning was done by hand after terminal bud set. The mean number of
fruits was 200, 120 and 50 per DC and 120, 80 and 30 per LC tree for the light, medium and heavy



Horticulturae 2019, 5, 0054 4 of 11

thinning treatments, respectively. The mean trunk cross-sectional area (0.6 m above graft union) was
13.37 cm2 and 13.74 cm2 for DC and LC trees, respectively.

The effect of storage duration on flesh color was quantified during 98 d of cold storage at 4 ◦C.

2.4. Data Analysis

All experiments were carried out with a minimum of 20 fruit sampled from a minimum of four
trees. Unless individual fruit data are shown, data are means ± standard errors. Where error bars are
not shown, they were smaller than the plotted symbols. Data were analyzed by analysis of variance
(Proc GLM) and regression analysis (Proc REG) using the statistical software package SAS (version
9.1.3; SAS Institute, Cary, NC, USA). Means were compared using Tukey’s Studentized Range (HSD)
Test. The significances of coefficients of determination (r2) at p ≤ 0.001 are indicated by ***.

3. Results

Absorption decreased exponentially as the L-value increased (Figure 2a). The curve had a
satisfactory resolution, i.e., changes in absorption resulted in measurable ∆L values over the entire range
of L-values. Plotting the natural log-transformed absorption vs. the L-value yielded a linear relationship.
For the a-value, absorption increased exponentially as the a-value increased (Figure 2b). However, the
curve segment for a-values from 30 to 50 was steep, thus the resolution was inferior to that in Figure 2a.
When taking the natural log of the absorption and plotting against the a-value, a linear relationship was
obtained between the two (Figure 2b, inset). Plots of absorption vs. the b-value yielded a discontinuous
curve with separate data populations for DC and LC (data not shown). The relationship between
the absorption of anthocyanins and the L-value (or a-value) determined using a spectrophotometer
allowed prediction of flesh color as indexed by anthocyanin content from measurements of the L-value
(or a-value) on a fruit cross-section. Plotting the predicted vs. measured anthocyanin absorption for
an independent data set yielded the relationships shown in Figure 2c. The absorption predicted from
L-values was closely and linearly related to the measured absorption (slope 1.12 ± 0.05, r2 = 0.98 ***).
The intercept did not differ significantly from zero and hence, the regression line was forced through
the origin. Relationships with the a-value were inferior, due to an overestimation of the predicted
absorption (slope 1.35 ± 0.13), systematic deviations for medium a-values (r2 = 0.93 ***).

Developmental increase in fruit size followed similar patterns in both clones (Figure 3a). The red
color of the flesh of the DC clone decreased slightly between 86 and 112 DAFB and then remained
constant until harvest (Figure 3b). In contrast, in the LC clone, the flesh began to color at 136 DAFB
and increased continuously in color intensity until 184 DAFB (Figure 3b). Compared with the LC
clone, the DC clone had a markedly higher percentage of dark- and medium-colored fruit (Figure 3c,d).
There was no relationship between the color of the skin or that of the outer or inner flesh in DC or LC
apples (data not shown).



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3. Results 

Absorption decreased exponentially as the L-value increased (Figure 2a). The curve had a 
satisfactory resolution, i.e., changes in absorption resulted in measurable ΔL values over the entire 
range of L-values. Plotting the natural log-transformed absorption vs. the L-value yielded a linear 
relationship. For the a-value, absorption increased exponentially as the a-value increased (Figure 
2b). However, the curve segment for a-values from 30 to 50 was steep, thus the resolution was 
inferior to that in Figure 2a. When taking the natural log of the absorption and plotting against the 
a-value, a linear relationship was obtained between the two (Figure 2b, inset). Plots of absorption vs. 
the b-value yielded a discontinuous curve with separate data populations for DC and LC (data not 
shown). The relationship between the absorption of anthocyanins and the L-value (or a-value) 
determined using a spectrophotometer allowed prediction of flesh color as indexed by anthocyanin 
content from measurements of the L-value (or a-value) on a fruit cross-section. Plotting the predicted 
vs. measured anthocyanin absorption for an independent data set yielded the relationships shown in 
Figure 2c. The absorption predicted from L-values was closely and linearly related to the measured 
absorption (slope 1.12 ± 0.05, r2 = 0.98 ***). The intercept did not differ significantly from zero and 
hence, the regression line was forced through the origin. Relationships with the a-value were 
inferior, due to an overestimation of the predicted absorption (slope 1.35 ± 0.13), systematic 
deviations for medium a-values (r2 = 0.93 ***). 

 
Figure 2. Absorption of anthocyanins extracted from the flesh of apples plotted against the color as 
indexed by the L-value (a) or the a-value (b). Each data point represents an individual tissue disc. 
Insets: Data from the main graph replotted, but absorption data ln transformed. (c) Relationship 
between the predicted absorption (Abspred) and the measured absorption (Absmeas). Absorption was 
predicted either from the L-value (Abspred = 1.12 (±0.05) × Absmeas + 0.78 (±0.37), r² = 0.98 ***) or from 
the a-values (Abspred = 1.35 (±0.13) × Absmeas + 5.08 (±0.89), r² = 0.93 ***). The L- and a-values were 
determined with a spectrophotometer in the L-, a- and b-modes. For details see text. 

Developmental increase in fruit size followed similar patterns in both clones (Figure 3a). The 
red color of the flesh of the DC clone decreased slightly between 86 and 112 DAFB and then 

Figure 2. Absorption of anthocyanins extracted from the flesh of apples plotted against the color as
indexed by the L-value (a) or the a-value (b). Each data point represents an individual tissue disc.
Insets: Data from the main graph replotted, but absorption data ln transformed. (c) Relationship
between the predicted absorption (Abspred) and the measured absorption (Absmeas). Absorption was
predicted either from the L-value (Abspred = 1.12 (±0.05) × Absmeas + 0.78 (±0.37), r

2 = 0.98 ***) or from
the a-values (Abspred = 1.35 (±0.13) × Absmeas + 5.08 (±0.89), r

2 = 0.93 ***). The L- and a-values were
determined with a spectrophotometer in the L-, a- and b-modes. For details see text.

Horticulturae 2019, 5, x FOR PEER REVIEW 5 of 10 

 

remained constant until harvest (Figure 3b). In contrast, in the LC clone, the flesh began to color at 
136 DAFB and increased continuously in color intensity until 184 DAFB (Figure 3b). Compared with 
the LC clone, the DC clone had a markedly higher percentage of dark- and medium-colored fruit 
(Figure 3c,d). There was no relationship between the color of the skin or that of the outer or inner 
flesh in DC or LC apples (data not shown). 

 
Figure 3. Developmental time course of change in diameter (a) and flesh color as indexed by the 
anthocyanin accumulation (b) in red flesh apples of a dark-colored (DC) and a light-colored (LC) 
clone. Distribution of color classes in DC (c) and LC clones (d). 

In both clones, flesh color intensity decreased from top to bottom positions in the tree crown 
(Figure 4a,b). The color distribution changed analogously (Figure 4c,d). Differences in sun exposure 
(north vs. south aspect) did not result in significant changes in flesh color (Figure 5). 

The intensity of flesh color decreased when branches were shaded with hail net (Figure 6a,b). 
UV-exposure did not affect flesh color in the DC clone (Figure 7a,c) but in the LC clone flesh color 
decreased significantly when fruit were covered with UV-absorbing film (Figure 7b,d).  

Compared with light fruit thinning, the medium and heavy fruit thinning both increased the 
red color in the flesh of both clones, DC and LC (Figure 8). 

There was no consistent change in flesh color during storage of either clone (Figure 9a). In the 
DC clone, an increasing proportion of fruit developed severe flesh browning as storage time 
increased. There was no browning in the LC clone (Figure 9b,c).  

Figure 3. Developmental time course of change in diameter (a) and flesh color as indexed by the
anthocyanin accumulation (b) in red flesh apples of a dark-colored (DC) and a light-colored (LC) clone.
Distribution of color classes in DC (c) and LC clones (d).



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In both clones, flesh color intensity decreased from top to bottom positions in the tree crown
(Figure 4a,b). The color distribution changed analogously (Figure 4c,d). Differences in sun exposure
(north vs. south aspect) did not result in significant changes in flesh color (Figure 5).Horticulturae 2019, 5, x FOR PEER REVIEW 6 of 10 

 

 
Figure 4. Effects of position along the central axis of a slender spindle tree on flesh anthocyanin 
content (a,b) and the color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a 
light-colored (LC) clone (b,d). 

 
Figure 5. Effects of the exposure of the fruit to the sun on flesh anthocyanin content (a,b) and the 
color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone 
(b,d). 

 

Figure 4. Effects of position along the central axis of a slender spindle tree on flesh anthocyanin content
(a,b) and the color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a light-colored
(LC) clone (b,d).

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Figure 4. Effects of position along the central axis of a slender spindle tree on flesh anthocyanin 
content (a,b) and the color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a 
light-colored (LC) clone (b,d). 

 
Figure 5. Effects of the exposure of the fruit to the sun on flesh anthocyanin content (a,b) and the 
color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone 
(b,d). 

 

Figure 5. Effects of the exposure of the fruit to the sun on flesh anthocyanin content (a,b) and the color
distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d).

The intensity of flesh color decreased when branches were shaded with hail net (Figure 6a,b).
UV-exposure did not affect flesh color in the DC clone (Figure 7a,c) but in the LC clone flesh color
decreased significantly when fruit were covered with UV-absorbing film (Figure 7b,d).



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Figure 4. Effects of position along the central axis of a slender spindle tree on flesh anthocyanin 
content (a,b) and the color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a 
light-colored (LC) clone (b,d). 

 
Figure 5. Effects of the exposure of the fruit to the sun on flesh anthocyanin content (a,b) and the 
color distribution (c,d) of red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone 
(b,d). 

 

Figure 6. Effects of shading on the anthocyanin content (a) and the color distribution (b) of red flesh
apples of a dark-colored (DC). Fruit exposed to full sunlight served as control. Shade reduced the
incident photosynthetically active radiation by 94%.

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Figure 6. Effects of shading on the anthocyanin content (a) and the color distribution (b) of red flesh 
apples of a dark-colored (DC). Fruit exposed to full sunlight served as control. Shade reduced the 
incident photosynthetically active radiation by 94%. 

 
Figure 7. Effect of UV radiation on the anthocyanin content (a,b) and the color distribution (c,d) of 
red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). UV radiation was 
excluded by wrapping the fruit in a bag made of UV-absorbing film. The film absorbed 100% of the 
UV radiation. Fruit that was exposed to full sunlight served as control. 

 
Figure 8. Effect of crop load on the anthocyanin content (a,b) and the color distribution (c,d) of red 
flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). Crop load was varied by 
hand thinning to different levels. The mean numbers of fruit per tree were 200, 120 and 50 per tree 
(DC) and 120, 80 and 30 per tree (LC) for the light, medium and heavy fruit thinning treatments, 
respectively. 

Figure 7. Effect of UV radiation on the anthocyanin content (a,b) and the color distribution (c,d) of
red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). UV radiation was
excluded by wrapping the fruit in a bag made of UV-absorbing film. The film absorbed 100% of the UV
radiation. Fruit that was exposed to full sunlight served as control.

Compared with light fruit thinning, the medium and heavy fruit thinning both increased the red
color in the flesh of both clones, DC and LC (Figure 8).



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Figure 6. Effects of shading on the anthocyanin content (a) and the color distribution (b) of red flesh 
apples of a dark-colored (DC). Fruit exposed to full sunlight served as control. Shade reduced the 
incident photosynthetically active radiation by 94%. 

 
Figure 7. Effect of UV radiation on the anthocyanin content (a,b) and the color distribution (c,d) of 
red flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). UV radiation was 
excluded by wrapping the fruit in a bag made of UV-absorbing film. The film absorbed 100% of the 
UV radiation. Fruit that was exposed to full sunlight served as control. 

 
Figure 8. Effect of crop load on the anthocyanin content (a,b) and the color distribution (c,d) of red 
flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). Crop load was varied by 
hand thinning to different levels. The mean numbers of fruit per tree were 200, 120 and 50 per tree 
(DC) and 120, 80 and 30 per tree (LC) for the light, medium and heavy fruit thinning treatments, 
respectively. 

Figure 8. Effect of crop load on the anthocyanin content (a,b) and the color distribution (c,d) of red
flesh apples of a dark-colored (DC) (a,c) and a light-colored (LC) clone (b,d). Crop load was varied by
hand thinning to different levels. The mean numbers of fruit per tree were 200, 120 and 50 per tree (DC)
and 120, 80 and 30 per tree (LC) for the light, medium and heavy fruit thinning treatments, respectively.

There was no consistent change in flesh color during storage of either clone (Figure 9a). In the DC
clone, an increasing proportion of fruit developed severe flesh browning as storage time increased.
There was no browning in the LC clone (Figure 9b,c).Horticulturae 2019, 5, x FOR PEER REVIEW 8 of 10 

 

 
Figure 9. Time course of change in the anthocyanin content (a) and the color distribution (b,c) of red 
flesh apples of a dark-colored (DC) (a,b) and a light-colored (LC) clone (a,c) during storage. Fruit 
were held for up to 96 days after harvest. 

4. Discussion 

Our experiments established two important findings: 1) the method of estimating anthocyanin 
content using calibrated photographs, image analysis and a spectrophotometer, proved reliable and 
sufficiently sensitive to quantify the effects of orchard management treatments imposed in field 
experiments, and 2) the effects of orchard management factors on anthocyanin biosynthesis were 
accounted for principally in terms of exposure to solar radiation. 

4.1. Quantifying Flesh Color Using Digital Photography and Image Analysis 

Measuring the redness of apple flesh based on digital photography and a calibration curve 
established between the L-value by a hand-held spectrophotometer and the anthocyanin absorption 
of flesh extract proved to be a quick, reliable and robust procedure for estimating flesh anthocyanin 
content. Compared to visual ratings, this method is more objective since it integrates spatial as well 
as color-intensity information, thereby producing a ’weighted’ redness. This is difficult to achieve 
using visual ratings, particularly when comparing flesh color assessed by different operators. For the 
two clones investigated, the accuracy of the procedure was excellent when based on measurements 
of L-value. It accounted for more than 98% of the variation in anthocyanin content measured in vitro. 
Furthermore, the slope of the regression line of predicted vs. measured anthocyanin content of an 
independent data set was 1.12 which is a slight and consistent overestimation of the measured 
anthocyanin content (r2 = 0.98).  

Interestingly, predictions of anthocyanin content based on the a-values were less accurate. This 
result is counterintuitive since the relationship of red coloration and the a-value on a red/green axis 
should be superior. We suggest the inaccuracy was due to insufficient resolution with the 
high-intensity red colorations, where the absorption of the extracts increased markedly for fairly 
small changes of a-value. 

4.2. Light Stimulation of Anthocyanin Biosynthesis 

Light was the common factor explaining the response of anthocyanin biosynthesis to the 
orchard management factors investigated. This was demonstrated in the observation that red color 
increased for fruit in the top of the crown, without shade by foliage or by covering by UV-absorbent 
film. These observations are consistent with those by Honda et al. (2017) [14] on different clones of 

Figure 9. Time course of change in the anthocyanin content (a) and the color distribution (b,c) of red
flesh apples of a dark-colored (DC) (a,b) and a light-colored (LC) clone (a,c) during storage. Fruit were
held for up to 96 days after harvest.

4. Discussion

Our experiments established two important findings: (1) the method of estimating anthocyanin
content using calibrated photographs, image analysis and a spectrophotometer, proved reliable and



Horticulturae 2019, 5, 0054 9 of 11

sufficiently sensitive to quantify the effects of orchard management treatments imposed in field
experiments, and (2) the effects of orchard management factors on anthocyanin biosynthesis were
accounted for principally in terms of exposure to solar radiation.

4.1. Quantifying Flesh Color Using Digital Photography and Image Analysis

Measuring the redness of apple flesh based on digital photography and a calibration curve
established between the L-value by a hand-held spectrophotometer and the anthocyanin absorption
of flesh extract proved to be a quick, reliable and robust procedure for estimating flesh anthocyanin
content. Compared to visual ratings, this method is more objective since it integrates spatial as well
as color-intensity information, thereby producing a ’weighted’ redness. This is difficult to achieve
using visual ratings, particularly when comparing flesh color assessed by different operators. For the
two clones investigated, the accuracy of the procedure was excellent when based on measurements of
L-value. It accounted for more than 98% of the variation in anthocyanin content measured in vitro.
Furthermore, the slope of the regression line of predicted vs. measured anthocyanin content of
an independent data set was 1.12 which is a slight and consistent overestimation of the measured
anthocyanin content (r2 = 0.98).

Interestingly, predictions of anthocyanin content based on the a-values were less accurate.
This result is counterintuitive since the relationship of red coloration and the a-value on a red/green axis
should be superior. We suggest the inaccuracy was due to insufficient resolution with the high-intensity
red colorations, where the absorption of the extracts increased markedly for fairly small changes
of a-value.

4.2. Light Stimulation of Anthocyanin Biosynthesis

Light was the common factor explaining the response of anthocyanin biosynthesis to the orchard
management factors investigated. This was demonstrated in the observation that red color increased
for fruit in the top of the crown, without shade by foliage or by covering by UV-absorbent film.
These observations are consistent with those by Honda et al. (2017) [14] on different clones of the same
two red-fleshed categories. They reported decreased anthocyanin concentration as crop load increased,
or for bagged vs. un-bagged fruit or for fruit grown in the shade vs. that exposed to the sun. Similarly,
Matsumoto et al. (2018) [15] found decreased red color in the outer flesh as indexed by the a-value
of the flesh when the fruit was shaded (by bagging), when crop load was high or when trees were
defoliated. When bags were removed, color intensity increased again in the outer flesh. They observed
no changes in the inner flesh [16]. Consistent with these reports was a decrease in anthocyanin content
when shaded of red-flesh and white-flesh clones of crab apple (Malus sylvestris) [7].

4.3. How Does Light Trigger Anthocyanin Biosynthesis in the Flesh?

There is little transmission through apple skin and parenchyma [17]. Thus, the question arises how
light triggers anthocyanin biosynthesis in the flesh of an apple when only the fruit surface is exposed
to light. Two hypotheses are offered that deserve investigation. First, anthocyanin biosynthesis may be
triggered by high concentrations of carbohydrates due to high rates of photosynthesis as a result of
high light exposure of the canopy. This hypothesis is consistent with the effects of crop load, shading
or defoliation observed in this and earlier studies [7,14,15].

Alternatively, photoreceptors may be considered. These perceive light levels at the fruit surface
and then—via some mobile agent—trigger anthocyanin biosynthesis in the flesh. That light triggers
anthocyanin biosynthesis is well established for the skin, for example in bagging experiments [14,16].
However, the flesh is not directly exposed. Blue light receptors (cryptochromes, phototropins) are
potential candidates because radiation of 450 nm wavelength stimulates blush in apple skins [18].
Cryptochrome MdCRY2 is known to regulate anthocyanin biosynthesis [19]. In strawberries (Fragaria
× ananassa Duch.), bio synthesis of anthocyanin is stimulated by 450 nm and by 730 nm wavelengths,



Horticulturae 2019, 5, 0054 10 of 11

the absorption maxima of phototropins and phytochromes (Pfr) [20]. Clearly, at this stage, the evidence
for a role of photoreceptors is not conclusive.

5. Conclusions

Digital photography plus image analysis is a quick and sufficiently precise method for quantifying
redness of the flesh of apples because it is closely related to anthocyanin content as determined in
the laboratory following extraction. The procedure is particularly useful because it does not require
sophisticated instruments and a laboratory setting. Although we investigated only two representatives
of the light- and dark-red flesh genotypes, we expect the relationship between anthocyanin absorption
and the L-value to also hold for other red-fleshed genotypes.

The results revealed that light is the most important environmental factor regulating anthocyanin
biosynthesis also in red flesh apple fruit. Increasing light exposure stimulated color development
under orchard conditions. Light exposure can be maximized by maintaining an open canopy structure,
pruning, thinning and by cultivating apples at sites with high levels of UV-B radiation.

Author Contributions: M.K. and E.G. designed the experiments; A.W. performed the experiments; A.W., E.G.,
M.K. analyzed the data; A.W. and E.G. prepared the draft of the paper; M.K. wrote the paper.

Funding: This research was funded in part by a grant from the IFORED group.

Acknowledgments: We thank Dirk Köpcke, Martin Brüggenwirth, Ulrich Hering, and Jennifer Kruse for their
support in setting up the experiments and Sandy Lang and Bishnu Khanal for helpful comments on an earlier
version of this manuscript.

Conflicts of Interest: The authors declare no conflict of interest.

References

1. Volz, R.K.; Oraguize, N.C.; Whitworth, C.J.; How, N.; Chagné, D.; Carlisle, C.M.; Gardiner, S.E.;
Rikkerink, E.H.A.; Lawrence, T. Red flesh breeding in apple: Progress and challenges. Acta Hortic. 2009, 814,
337–342. [CrossRef]

2. Van Nocker, S.; Berry, G.; Najdowski, J.; Michelutti, R.; Luffman, M.; Forsline, P.; Alsmairat, N.; Beaudry, R.;
Nair, M.G.; Ordidge, M. Genetic diversity of red-fleshed apples (Malus). Euphytica 2012, 185, 281–293.
[CrossRef]

3. Contessa, C.; Botta, R. Comparison of physiochemical traits of red-fleshed, commercial and ancient apple
cultivars. Hortic. Sci. 2016, 43, 159–166. [CrossRef]

4. Espley, R.V.; Hellens, R.P.; Putterill, J.; Stevenson, D.E.; Kutty-Amma, S.; Allan, A.C. Red colouration in apple
fruits is due to the activity of the MYB transcription factor, MdMYB10. Plant J. 2007, 49, 414–427. [CrossRef]
[PubMed]

5. Chagné, D.; Lin-Wang, K.; Espley, R.V.; Volz, R.K.; How, N.M.; Rouse, S.; Brendolise, C.; Carlisle, C.M.;
Kumar, S.; De Silva, N.; et al. An ancient duplication of apple MYB transcription factors is responsible for
novel red fruit-flesh phenotypes. Plant Physiol. 2013, 161, 225–239. [CrossRef] [PubMed]

6. Umemura, H.; Otagaki, S.; Wada, M.; Kondo, S.; Matsumoto, S. Expression and functional analysis of a novel
MYB gene, MdMYB110a_JP, responsible for red flesh, not skin color in apple fruit. Planta 2013, 238, 65–76.
[CrossRef] [PubMed]

7. Wang, Y.; Lu, Y.; Hao, S.; Zhang, M.; Zhang, J.; Tian, J.; Yao, Y. Different coloration patterns between the red-
and white-fleshed fruits of malus crabapples. Sci. Hortic. 2015, 194, 26–33. [CrossRef]

8. He, J.; Giusti, M.M. Anthocyanins: Natural colorants with health-promoting properties. Ann. Rev. Food
Sci. Technol. 2010, 1, 163–187. [CrossRef] [PubMed]

9. Mazza, G.; Miniati, E. Anthocyanins in Fruits, Vegetables, and Grains, 1st ed.; CRC Press: Boca Raton, FL,
USA, 1993.

10. Zhang, Y.; Zhao, R.; Liu, W.; Sun, X.; Bai, S.; Xiang, Y.; Dai, H. The anthocyanins component and the influence
factors of contents in red flesh apple ‘Hong-Xun No. 1’. Eur. J. Hortic. Sci. 2016, 81, 248–254. [CrossRef]

11. Musacchi, S.; Serra, S. Apple fruit quality: Overview on pre-harvest factors. Sci. Hortic. 2018, 234, 409–430.
[CrossRef]

http://dx.doi.org/10.17660/ActaHortic.2009.814.54
http://dx.doi.org/10.1007/s10681-011-0579-7
http://dx.doi.org/10.17221/132/2015-HORTSCI
http://dx.doi.org/10.1111/j.1365-313X.2006.02964.x
http://www.ncbi.nlm.nih.gov/pubmed/17181777
http://dx.doi.org/10.1104/pp.112.206771
http://www.ncbi.nlm.nih.gov/pubmed/23096157
http://dx.doi.org/10.1007/s00425-013-1875-3
http://www.ncbi.nlm.nih.gov/pubmed/23568403
http://dx.doi.org/10.1016/j.scienta.2015.07.041
http://dx.doi.org/10.1146/annurev.food.080708.100754
http://www.ncbi.nlm.nih.gov/pubmed/22129334
http://dx.doi.org/10.17660/eJHS.2016/81.5.3
http://dx.doi.org/10.1016/j.scienta.2017.12.057


Horticulturae 2019, 5, 0054 11 of 11

12. Honda, C.; Moriya, S. Anthocyanin biosynthesis in apple fruit. Hortic. J. 2018, 87, 305–314. [CrossRef]
13. McGuire, R.G. Reporting of objective color measurements. HortScience 1992, 27, 1254–1255. [CrossRef]
14. Honda, C.; Iwanami, H.; Naramoto, K.; Maejima, T.; Kanamaru, K.; Moriya-Tanaka, Y.; Hanada, T.; Wada, M.

Thinning and bagging treatments and the growing region influence anthocyanin accumulation in redfleshed
apple fruit. Hortic. J. 2017, 86, 291–299. [CrossRef]

15. Matsumoto, K.; Fujita, T.; Sato, S.; Moriguchi, T. Effects of low temperature, shading, defoliation, and crop
load on the flesh coloration of the type 2 red-fleshed apple ‘Kurenainoyume’. Hortic. J. 2018, 87, 452–461.
[CrossRef]

16. Matsumoto, K.; Kobayashi, T.; Kuogo, T.; Fujita, T.; Sato, S.; Moriguchi, T. Sunlight differentially affects the
fruit skin, flesh, and core coloration of the type 2 re-fleshed apple ‘Kurenainoyume’: Optimization of fruit
bagging treatment. Hortic. J. 2018, 87, 462–473. [CrossRef]

17. Blanke, M.M.; Notton, B.A. Light transmission into apple fruit and leaves. Sci. Hortic. 1992, 51, 43–53.
[CrossRef]

18. Arakawa, O.; Kikuya, S.; Pungpomin, P.; Zhang, S.; Tanaka, N. Accumulation of anthocyanin in apples in
response to blue light at 450 nm: Recommendations for producing quality fruit color under global warming.
Eur. J. Hortic. Sci. 2016, 81, 297–302. [CrossRef]

19. Li, Y.; Mao, K.; Zhao, C.; Zhao, X.; Zhang, R.; Zhang, H.; Shu, H.; Hao, Y. Molecular cloning and functional
analysis of a blue light receptor gene MdCRY2 from apple (Malus domestica). Plant Cell Rep. 2013, 32, 555–566.
[CrossRef] [PubMed]

20. Zhang, Y.; Jiang, L.; Li, Y.; Chen, Q.; Ye, Y.; Zhang, Y.; Luo, Y.; Wang, X.; Tang, H. Effect of red and blue light
on anthocyanin accumulation and differential gene expression in strawberry (Fragaria × ananassa). Molecules
2018, 23, 820. [CrossRef] [PubMed]

© 2019 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access
article distributed under the terms and conditions of the Creative Commons Attribution
(CC BY) license (http://creativecommons.org/licenses/by/4.0/).

http://dx.doi.org/10.2503/hortj.OKD-R01
http://dx.doi.org/10.21273/HORTSCI.27.12.1254
http://dx.doi.org/10.2503/hortj.OKD-010
http://dx.doi.org/10.2503/hortj.OKD-130
http://dx.doi.org/10.2503/hortj.OKD-120
http://dx.doi.org/10.1016/0304-4238(92)90102-I
http://dx.doi.org/10.17660/eJHS.2016/81.6.2
http://dx.doi.org/10.1007/s00299-013-1387-4
http://www.ncbi.nlm.nih.gov/pubmed/23314496
http://dx.doi.org/10.3390/molecules23040820
http://www.ncbi.nlm.nih.gov/pubmed/29614032
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http://creativecommons.org/licenses/by/4.0/.

	Introduction 
	Materials and Methods 
	Plant Material 
	Quantifying Redness of Cross-Sections 
	Experiments 
	Data Analysis 

	Results 
	Discussion 
	Quantifying Flesh Color Using Digital Photography and Image Analysis 
	Light Stimulation of Anthocyanin Biosynthesis 
	How Does Light Trigger Anthocyanin Biosynthesis in the Flesh? 

	Conclusions 
	References