1/8Brazilian Journal of Biology, 2024, vol. 84, e253436 | https://doi.org/10.1590/1519-6984.253436

Original Article

THE INTERNATIONAL JOURNAL ON NEOTROPICAL BIOLOGY
THE INTERNATIONAL JOURNAL ON GLOBAL BIODIVERSITY AND ENVIRONMENT

ISSN 1519-6984 (Print)
ISSN 1678-4375 (Online)

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, 
distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract
The in vitro sporulation of Didymella bryoniae is of great importance for studies that require pure inoculum and in 
large quantities. Thus, the objectives of this study were to identify the best condition for D. bryoniae sporulation 
combining different light spectra (UV-A or UV-B light, white light, and continuous dark), with distinct culture media 
(PDA, V8, ML, and PDAB) and, to evaluate fungus’ survivability stored at -20°C over time. The fungus samples were 
only able to sporulate when subjected to the UV-B light treatment, regardless of the culture medium. The highest 
appearance of spores conidium type was observed in the PDAB medium, and the lowest production occurred in 
the ML medium. Reproductive structures, such as perithecia and pycnidia, were observed in all culture media. 
However, there was considerable variation in the amount of each structure between the different culture media. 
The ML and V8 media showed a greater number of perithecia and the PDA and PDAB media presented a greater 
proportion of pycnidia compared to perithecia. The storage duration at -20°C did not affect mycelial growth or 
mycelial growth rate. In conclusion, the UV-B light is essential for D. bryoniae in vitro sporulation. Moreover, 
the culture medium composition influences the type of fungal structure produced, as well as spores’ size and 
quantity. Freezing at -20°C is an efficient technique that can be used to store D. bryoniae for at least five months 
without loss of viability.

Keywords: fungi preservation, gummy stem blight, sporulation, UV-B light.

Resumo
A esporulação de Didymella bryoniae in vitro é de grande importância para estudos que requerem inóculo puro e em 
grandes quantidades. Assim, os objetivos deste estudo foram identificar a melhor condição para esporulação de D. 
bryoniae combinando diferentes espectros de luz (luz UV-A ou UV-B, luz branca e escuro contínuo) com distintos 
meios de cultura (PDA, V8, ML e PDAB) e, avaliar a sobrevivência do fungo armazenado a -20°C ao longo do tempo. 
As amostras de fungo só esporularam quando submetidas ao tratamento com luz UV-B, independentemente do 
meio de cultura. Maior aparecimento de esporos do tipo conídio foi observado no meio PDAB, e a menor produção 
ocorreu no meio ML. Estruturas reprodutivas, como peritécios e picnídeos, foram observadas em todos os meios de 
cultura. No entanto, houve uma variação considerável na quantidade de cada estrutura entre os diferentes meios de 
cultura. Os meios ML e V8 apresentaram maior número de peritécios e os meios PDA e PDAB apresentaram maior 
proporção de picnídeos em relação aos peritécios. A duração do armazenamento a -20°C não afetou o crescimento 
micelial ou a taxa de crescimento micelial. Em conclusão, a luz UV-B é essencial para a esporulação de D. bryoniae 
in vitro. Além disso, a composição do meio de cultura influencia o tipo de estrutura fúngica produzida, bem como 
o tamanho e a quantidade dos esporos. O congelamento a -20°C é uma técnica eficiente que pode ser usada para 
armazenar D. bryoniae por pelo menos cinco meses sem perda de viabilidade

Palavras-chave: Preservação de fungos, crestamento gomoso do caule, esporulação, Luz UV-B.

Providing inoculum for Didymella bryoniae studies: the effect 
of light spectrum and storing at low temperature
Fornecendo inóculo para estudos de Didymella bryoniae: o efeito do espectro de luz e 
armazenamento em baixa temperatura

M. C. S. Virtuosoa* , E. H. C. Silvab , E. M. Silvaa , T. S. Valentec,d , P. F. Vargase , L. T. Braze  and R. C. Panizzie 
aUniversidade Estadual Paulista – UNESP, Faculdade de Ciências Agrárias e Veterinárias, Programa de Pós-graduação em Agronomia (Genética e 
Melhoramento de Plantas), Jaboticabal, SP, Brasil

bInstituto Taquaritinguense de Ensino Superior “Dr. Aristides de Carvalho Schlobach” – ITES, Departamento de Agronomia, Taquaritinga, SP, 
Brasil

cUniversity of Alberta – UAlberta, Department of Agricultural, Food and Nutritional Science, Edmonton, Canada
dUniversidade Estadual Paulista – UNESP, Faculdade de Ciências Agrárias e Veterinárias, Departamento de Zootecnia, Jaboticabal, SP, Brasil
eUniversidade Estadual Paulista – UNESP, Faculdade de Ciências Agrárias e Veterinárias, Departamento de Ciências da Produção Agrícola, 
Jaboticabal, SP, Brasil

*e-mail: marcos.virtuoso@unesp.br
Received: June 18, 2021 – Accepted: September 30, 2021

https://creativecommons.org/licenses/by/4.0/
https://orcid.org/0000-0002-9142-273X
https://orcid.org/0000-0002-3554-4118
https://orcid.org/0000-0002-3196-6516
https://orcid.org/0000-0003-2418-154X
https://orcid.org/0000-0002-5718-6403
https://orcid.org/0000-0003-1420-0364
https://orcid.org/0000-0002-0289-6563


Brazilian Journal of Biology, 2024, vol. 84, e2534362/8

Virtuoso, M.C.S. et al.

at -20°C for the storage of D. bryoniae isolates. However, 
these authors did not carry out systematic evaluations 
to verify the preservation and survival of the fungus over 
time, nor of its structures. Thus, little is known about the 
survival capacity of D. bryoniae stored at low temperatures.

Based on the above considerations, there is a need 
to establish the ideal condition for in vitro D. bryoniae 
sporulation, as well as to evaluate the survival capacity 
of this fungus when stored at low temperature. Thus, 
the objectives of the present study were to establish the 
best condition for D. bryoniae sporulation combining 
different light spectra and culture media, and to evaluate 
the fungus’ ability to survive over time when submitted 
to the -20°C storage.

2. Material and Methods

The present study was carried out at São Paulo State 
University, School of Agricultural and Veterinarian Sciences, 
Jaboticabal Campus (21°15′19″S, 48°19′21″ O), São Paulo - 
Brazil. Melon plants (Cucumis melo L.) with symptoms of 
GSB, such as the presence of viscous exudate and fruiting 
bodies of the fungus, were used to obtain the D. bryoniae 
isolate. The pycnidia/perithecium were directly removed 
from lesions on the stem was performed with the aid of 
a magnifying glass. These structures were placed in Petri 
dishes containing PDA (potato-dextrose-agar) medium, 
subsequently closed with PVC film, and incubated in 
growth chambers, with a constant temperature of 24°C 
and a 12-hour photoperiod for 4 consecutive days. After 
obtaining the fungal culture, a subculture was carried out 
to purify the fungus, transferring 5 mm diameter discs 
with mycelium to new plates and conditioning them for 
10 days, forming the stock cultures.

The study was conducted in two stages to assess 
the ability of in vitro sporulation and survival after 
freezing. In the first phase of the study, a completely 
randomized design was used in a 4 x 4 factorial scheme 
with 10 repetitions, the factors being represented by the 
different culture media and types of light. In the second 
phase, the growth capacity was evaluated after different 
periods of freezing at -20°C.

2.1. Culture medium and light spectrum

To evaluate the sporulation capacity of D. bryoniae, four 
culture media were used, namely: i) potato-dextrose-agar 
(PDA), ii) concentrated vegetable juice (V8, commercial 
product), iii) melon leaf extract (ML), and iv) potato-
dextrose-agar + melon branches (PDAB). In addition, 
four light spectra were used, being: i) white fluorescent 
light 440-740 nm/10W, ii) UV-A white fluorescent light, 
350-400 nm/8W, iii) UV-B white fluorescent light, 
280-360 nm/8W, and iv) control group in continuous dark.

PDA and PDAB culture media were prepared with 200g 
of potatoes chopped into small cubes and placed in 1.0 L 
of deionized water and cooked at 100°C for 20 minutes. 
To the potato extract, 20 g of dextrose and 20 g of agar 
were added, completing the volume with deionized water 
to 1.0 L. For the preparation of the V8 medium, 20 g of 
agar was added to 200 mL of concentrated vegetable 
juice, then the volume was adjusted to 1.0 L, and finally, 

1. Introduction

The Didymella bryoniae (Auersw.) Rehm, synonym 
Stagonosporopsis cucurbitacearum (Fr.) [anamorph Phoma 
cucurbitacearum (Fr.) Sacc (=Ascochyta cucumis Fautrey & 
Roum)] (Mao et al., 2020), is an ascomycete that causes 
the gummy stem blight (GSB) in several cucurbits. 
When present in cucurbits cultures this fungus might 
negatively impact yield with direct consequent economic 
revenue decreases for growers (Liu et al., 2017). Given 
the importance of D. bryoniae, studies involving in vitro 
cultivation and sporulation are relevant, especially when 
a large amount of pure inoculum is needed. For example, 
screening for resistant plants requires a high number of 
spores to guarantee the intensity of the disease. Moreover, 
GSB-related studies often require the combination of 
inoculations in a greenhouse and subsequent field tests 
(Gusmini et al., 2003).

To date, several studies evaluating the best condition 
for D. bryoniae sporulation in vitro have been reported, 
testing different culture medium (CM) combinations 
(Gusmini et al., 2003; Hassan et al., 2018; Leão et al., 
2012; Nga et al., 2010; Skarshaug, 1981; Somai et al., 
2002), ultraviolet (UV) light (Kwon et al., 1997; Lee, 1982; 
Tsay et al., 1990; Tsutsumi and Silva, 2004; Wolukau et al., 
2007; Zhang et al., 2017), and temperature and pH 
(Bhat et al., 2009). However, despite the vast literature on 
the subject, there is still no consensus among researchers on 
the main factors influencing in vitro D. bryoniae sporulation, 
with frequent disagreement between studies.

According to Keinath et al. (1995) and Wiant (1945), 
some isolates do not sporulate in any CM. On the other 
hand, Leão et al. (2012) observed that the CM can influence 
D. bryoniae sporulation. In addition, Choi et al. (2010) and 
Kwon et al. (1997) concluded that the presence of UV light 
is important to promote the sporulation of this fungus. 
Despite the direct effect that UV light may have on D. 
bryoniae sporulation, many studies do not classify the type 
of UV used, hampering the use of a similar methodology. 
Such information is important because UV lights can be 
classified according to the emitted wavelength, being UV-A 
(315–400 nm), UV-B (280–315 nm), or UV-C (100–280 nm) 
(Braga et al., 2015).

In addition to the CM and the type of light, the 
storage time is also important for the development of 
research with D. bryoniae. Properly stored samples serve 
as quick-access natural resources banks, which can be 
used for the development of studies on biodiversity, 
systematics, phytopathology, and related areas, such as 
plant breeding for resistance to diseases (Aparecido et al., 
2018; Hawksworth and Colwell 1992; Sakr, 2019). The most 
used methods for fungi preservation are submersion in 
sterile water, mineral oil, or glycerol, use of filter paper 
discs, wood, soil, and silica gel (Al-Bedak et al., 2019). Also, 
cryopreservation, lyophilization, and preservation under 
liquid nitrogen can be employed (Ayala-Zermeño et al., 
2017).

Freezing at -20°C has also been shown to be a safe 
method for storing various microorganisms and, unlike 
cryopreservation and preservation under liquid nitrogen, 
which requires more sophisticated equipment, storing at 
-20°C is simple and of low cost (Tortora et al., 2011). To the 
best of our knowledge, only Grube et al. (2011) used freezing 



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Providing inoculum for Didymella bryoniae studies

3.2 g of CaCO3 was added to raise the pH to 7.0. For the ML 
medium, 200g of melon leaves were washed in running 
water and then processed in a blender with 500mL of 
deionized water, then sieved twice in non-woven fabrics 
(TNT) and then added with 20g of agar and 20g of dextrose, 
completing the process. volume to 1.0 L. The pH of all 
culture media was assessed and, when necessary, adjusted 
to standardize at 7.0.

After preparation, all culture media were sterilized 
by autoclaving for 20 minutes at 121ºC, then 200 mg 
of antibiotic (streptomycin) was added. Subsequently, 
5 mL of each medium was poured into test tubes (14.5 x 
2.5 cm). In this step, three pieces of 5 cm melon branches 
were added to the PDAB medium, previously disinfected 
in 1% bleach, and dried on filter paper. Finally, the tubes 
were covered with cotton, sealed with aluminum foil, and 
again autoclaved.

At the beginning of the experiment, 5 mm diameter 
discs with mycelium of the fungus were removed from 
the stock plates and transferred to the center of each 
test tube. Subsequently, the tubes were incubated in a 
growth chamber with a constant temperature of 24°C and 
subjected to a photoperiod of 16 hours of light, except for 
the continuous dark treatment, for 20 consecutive days. 
During this photoperiod, all tubes were placed 20 cm away 
from the lamps allowing maximum possible radiation.

The spore concentration was determined for 
all treatments after 20 days of incubation, using a 
hemacytometer. For the solution preparation, the culture 
medium was removed from the tube and placed in a 
crucible with 20 mL of sterile water, then macerated to 
release the spores. After maceration, filtration in voile 
tissue was carried out to remove remnants of the culture 
medium and mycelium, followed by the addition of 0.2% 
Tween 20. The results were expressed as number of 
spores per mL. In addition, the mycelium staining, type of 
sexual structures (perithecia and pycnidia), and the spore 
morphology were visually evaluated with the aid of an 
optical microscope with an attached camera (Olympus 
cellSens standard 2.3). The morphological classification 
of spores followed the methodology proposed by Chiu 
and Walker (1949).

2.2. Storing at -20°C

To verify fungal survivability after different periods 
of storing at -20°C, a completely randomized design 
was employed, considering the storage time (in months) 
as treatment, with five repetitions. Following the 
aforementioned methodology, PDAB tubes were prepared 
and then conditioned in the growth chamber under UV-B 
light to sporulate. After the fungus had sporulated, tubes 
were taken to a freezer (-20°C) and stored for up to five 
consecutive months.

A tube of PDAB medium was removed from the freezer 
every 30 days of storage to obtain D. bryoniae fungal 
structures. These samples were transferred to five Petri 
dishes containing PDA medium, which were sealed with 
plastic film and incubated in a growth chamber at a 
constant temperature of 24ºC, with a 12-hour photoperiod 
and white fluorescent light regime.

In this phase, daily evaluations of mycelial growth were 
performed, measuring two diametrically opposite points of 

the colony perimeter, discounting 10.0 mm corresponding 
to the initial inoculum of the fungus, for five consecutive 
days. The data were used to calculate the average mycelial 
growth at five days and to obtain the mycelial growth rate 
index (MGRI), using the method proposed by Maia et al. 
(2011), as follow (Equation 1):

( ) 
 aD D

MGRI
N

∑ −
=  (1)

where D  is the current average diameter of the colony, 
aD  is the average diameter of the colony of the previous 

day, and N  is the number of days of evaluation.

2.3. Statistical analysis

The spore concentration data were transformed to 
root(x) and subjected to analysis of variance and comparison 
of means by the Tukey test (Tukey, 1953). The data 
relating to AG and MGRI were submitted to analysis of 
variance. The analyzes were performed using software R 
(R Development Core Team, 2018).

3. Results

There was no significant interaction between the 
culture medium and the type of light used to promote 
in vitro sporulation of D. bryoniae. The fungus samples 
were only able to sporulate when subjected to the UV-B 
light treatment, regardless of the culture medium. 
The other light conditions did not cause any stimulus to 
sporulation, or even traces of reproductive structures. 
As a result, comparisons using the mean test were only 
performed between different culture media under UV-B 
light treatment and, a significant difference was observed 
for the number of spores among the four culture medium 
evaluated (P<0.001). The highest appearance of spores 
conidium type was observed in the PDAB medium, and the 
lowest production occurred in the ML medium (Figure 1).

Figure 1. Average conidia concentration of Didymella bryoniae 
produced in different culture media under UV-B light. PDA = potato-
dextrose-agar; PDAB = potato-dextrose-agar + melon branches; 
V8 = concentrated vegetable juice (commercial); ML = melon 
leaf extract.



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Virtuoso, M.C.S. et al.

Reproductive structures, such as perithecia and pycnidia, 
were observed in all culture media. However, there was 
considerable variation in the amount of each structure 
between the different culture media used as shown in 
Table 1. The ML and V8 media showed a greater number 
of perithecia in relation to the pycnidia. This variation 
might have influenced the final spore count since, despite 
a large number of structures the ascospores are difficult 
to visualize on the hemacytometer, resulting in reduced 
total spores’ count. In contrast, the PDA and PDAB media 
presented a greater proportion of pycnidia compared 
to perithecia, resulting in a higher conidia appearance 
(Figure 1). It worth mentioning the importance of PDAB 
medium to promote pycnidia production since most of the 
formed structures were present in the melon branches.

The visual analysis employed for mycelium 
characterization indicated that the light type is an important 
factor affecting both the appearance and color of the fungus’ 

structures. When submitted to growth in UV-B light, the 
mycelium showed a darker color (dark gray) compared 
to all other evaluated light conditions. Samples subjected 
to continuous dark, or UV-A light presented white color, 
and those under fluorescent light were greyish-white. 
In addition, it was observed that the mycelium volume 
is smaller when subjected to UV-B light but with a larger 
number of perithecia and pycnidia (Figure 2).

Regarding morphological aspects evaluated, the 
appearance of septate and non-septate conidia was 
observed in all culture media under UV-B light as shown 
in Figure 3A. However, an important size variation was 
observed in which the largest microconidium production 
occurred in the V8 medium, with structure size ranging 
from 3 to 5 µm. In the other culture media, there were a 
higher proportion of macroconidia, ranging from 6 to 10 µm 
in length according to the classification proposed by Chiu 
and Walker (1949). Moreover, in all assessed media the 
asci’s size ranged from 35 to 50 µm and the ascospores 
from 6.5 to 12 µm in length (Figure 3B).

As greater D. bryoniae sporulation was observed in 
samples submitted to PDAB medium and under UV-B light, 
this treatment was used to produce biological material for 
further freezing. At this stage of the experiment, the fungus 
survivability was evaluated after different storage periods 
at -20°C. However, there was no significant difference 
(P>0.05) between the freezing times on mycelial growth 
and the mycelial growth rate index (Figure 4). This result 
indicates that when subjected to a combination of PDAB 
medium with UV-B light, the fungus can survive, and 
biological functions are preserved after freezing at -20°C 
for up to five months.

Table 1. Spores of Didymella bryoniae produced in different media 
under UV-B light.

Culture mediaa Perithecia Pycnidia

PDAB ++ ++++

PDA ++ +++

V8 +++ ++

ML ++++ +

+ = scarce; ++ = moderate; +++ = good; ++++ = abundant.  aPDAB = potato-
dextrose-agar + melon branches; PDA = potato-dextrose-agar; 
V8 = concentrated vegetable juice (commercial); ML = melon leaf extract.

Figure 2. Characteristics of Didymella bryoniae reproductive structures in vitro. (A) PDAB medium = potato-dextrose-agar + melon 
branches, (B) on the branch; and (C) on the medium.



Brazilian Journal of Biology, 2024, vol. 84, e253436 5/8

Providing inoculum for Didymella bryoniae studies

4. Discussion

The results obtained in our study showed that regardless 
of the culture medium, the in vitro sporulation of Didymella 
bryoniae isolate occurs only in the presence of ultraviolet 
radiation, more specifically, the light spectrum in the 
wavelength between 280-360 nm (peaking at 315nm). 
According to Sepúlveda et al. (2009), some photoreceptors 
are only activated when stimulated by light with specific 
wavelengths. In addition, other authors reported that in 
several species the light has a regulatory effect on the 
development and behavior of fungi (Corrochano, 2007; 
Pulz and Massola Jr., 2009).

The quality and intensity of light are also important 
aspects to promote in vitro sporulation of D. bryoniae. 

During preliminary tests (unpublished data), it was possible 
to stimulate the formation of reproductive structures 
when using a 12-hour photoperiod with tubes placed 
25 cm away from the lights, however, sporogenesis or 
spore maturation did not occur. Chiu and Walker (1949) 
also observed the formation of reproductive structures 
without the presence of spores. These authors report that 
the absence of sporulation on the material used occurred 
due to specific nutritional requirements by the different 
isolates of D. bryoniae. Considering that in the natural 
environment the fungus receives appropriate quality 
and amount of light to sporulate, these factors (number 
of light hours, intensity, and spectrum) are key elements 
that need to be considered under laboratory conditions 
to promote satisfactory sporulation of this fungi.

Figure 3. (A) Conidia of the imperfect form of Didymella bryoniae; (B) Asci and ascospores of the perfect form of Didymella bryoniae 
(100x amplification, scale = 10µm).

Figure 4. Average values of mycelial growth (A) and mycelial growth rate index (B) for the Didymella bryoniae fungus stored over five 
consecutive months at -20° C.



Brazilian Journal of Biology, 2024, vol. 84, e2534366/8

Virtuoso, M.C.S. et al.

During the first phase of the experiment, the appearance 
of reproductive structures occurred both on the surface 
and submerged in the culture medium, which is why 
maceration was defined as the best method for obtaining 
the spores produced. Similar behavior was observed by 
Leach (1962) when working with the sporulation of the 
fungus Ascochyta pisi. During preliminary evaluations, it 
was observed that the sporulation induction occurred in 
young mycelia only, soon after their exposure to UV-B 
light. On the other hand, there was no induction when 
mature mycelia were placed under UV-B light (personal 
communication). Leach (1962) also reported that young 
mycelium is more sensitive to UV light radiation acting 
as a receptor compared to mature mycelium.

The fungal structure type formed varied among the 
four media used (Table 1). The ML medium showed higher 
production of perithecia than pycnidia, indicating that 
there is a higher occurrence of sexual reproduction in this 
medium caused by the greater availability of essential 
substances for fungus development. The greater appearance 
of perithecia might be explained by the fact that sexual 
reproduction has higher physiological requirements 
and energy costs compared with asexual reproduction 
(Chamberlain and Ingram, 1997). Conversely, in other media 
(PDA, PDAB, and V8) there is less availability of nutritional 
resources with consequently increased occurrence of 
asexual reproduction. These results partially corroborate 
Lee (1982), who obtained different sexual structures of D. 
bryoniae when submitted to PDA, V8, and plant extracts. 
However, this author attributed the observed differences 
to the origin of their isolates. In practical terms, the PDAB 
medium is more suitable to be used when screening 
to identify resistant plants, since the pycnidiospores 
produced are more easily visualized and quantified on 
a hemacytometer. On the other hand, the ML medium is 
mainly indicated to study genetic aspects of this fungus.

In addition to the influence on the development 
of reproductive structures, the medium composition 
also proved to be a determining factor for the size of 
pycnidiospores. In the V8 medium, there was a higher 
proportion of microconidia compared to all other media. 
In this case, the carbon source may be responsible for the 
variation observed in spore size, given that the V8 medium 
is the only that dextrose was not added. Similar results 
were observed by Chiu and Walker (1949) and Lee (1982) 
who associated the conidia size to the type of medium 
and isolate used.

Regarding the fungus’ ability to survive after freezing 
at -20°C, there was no significant difference in average 
mycelial growth and mycelial growth rate index among 
the five different periods of freezing as presented in 
Figure 4 (P>0.05). This result indicates that the D. bryoniae 
can be stored at low temperatures, maintaining a high 
ability of survival and growth rate over time. According 
to Ayala-Zermeño et al. (2017), freezing significantly 
reduces cellular metabolism, keeping the fungus viable for 
long periods. Thus, the high viability in the last month of 
evaluation (Figure 4) suggests that the fungus can remain 
viable for longer periods than those evaluated in the 
present study, without significant damage. It is important 
to highlight that, because of the experimental design it 

was not possible to systematically assess survivability 
after five months and, thus, further studies are required 
to improve our knowledge on this behalf.

Another important aspect that should be highlighted 
is the fact that the freezing was carried out using the 
PDAB medium, which biological material contains a high 
concentration of fungal spores. According to Meryman 
(1966) and Sakr (2019) spores, sclerotia, and dormant 
mycelium are the most resistant fungal structures to 
freezing because their cells have less moisture content. 
On the other hand, cellular structures with a higher 
moisture content tend to be more susceptible to damage 
caused by low temperatures.

To the best of our knowledge, to date, no studies have 
been developed to identify the main factors related to in 
vitro sporulation of D. bryoniae neither its ability to survive 
after freezing. Our results showed that it is possible to 
stimulate the sporulation of this fungus in vitro and that 
approachable techniques can be used for the storage and 
conservation of biological material.

In conclusion, this is the first study identifying 
key elements of light and culture medium affecting 
the Didymella bryoniae in vitro sporulation and the 
consequences of freezing during five consecutive months. 
The spectrum emitted by UV-B light is the main factor 
promoting in vitro sporulation. Moreover, the culture 
medium composition influences the type of fungal structure 
produced, as well as spores’ size and quantity. Freezing at 
-20°C is an efficient technique that can be used to store D. 
bryoniae for at least five months without loss of viability.

Acknowledgements

This study was financed in part by the Coordenação 
de Aperfeiçoamento de Pessoal de Nível Superior - Brasil 
(CAPES) - Finance Code 001, which had no role in study 
design, data collection and analysis, decision to publish, or 
preparation of the manuscript. The study was part of the 
doctoral thesis of the first author, prepared for the Graduate 
Program in Genetics and Plant Breeding at Universidade 
Estadual Paulista (UNESP), Faculdade de Ciências Agrárias 
e Veterinárias, Jaboticabal, SP, Brasil.

References

AL-BEDAK, O.A., SAYED, R.M. and HASSAN, S.H.A., 2019. A new 
low-cost method for long-term preservation of filamentous 
fungi. Biocatalysis and Agricultural Biotechnology, vol. 22, no. 
11, pp. 101417. http://dx.doi.org/10.1016/j.bcab.2019.101417.

APARECIDO, C.C., ROSA, E.C., COSTA, I.A.M. and JORGE, C.M., 2018. 
Avaliação de diferentes métodos para preservação de fungos 
fitopatogênicos. O Biológico, vol. 80, no. 1, pp. 1-7.

AYALA-ZERMEÑO, M.A., GALLOU, A., BERLANGA-PADILLA, A.M., 
ANDRADE-MICHEL, G.Y., RODRÍGUEZ-RODRÍGUEZ, J.C., 
ARREDONDO-BERNAL, H.C. and MONTESINOS-MATÍAS, R., 2017. 
Viability, purity, and genetic stability of entomopathogenic 
fungi species using different preservation methods. Fungal 
Biology, vol. 121, no. 11, pp. 920-928. http://dx.doi.org/10.1016/j.
funbio.2017.07.007. PMid:29029699.

https://doi.org/10.1016/j.bcab.2019.101417
https://doi.org/10.1016/j.funbio.2017.07.007
https://doi.org/10.1016/j.funbio.2017.07.007
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=29029699&dopt=Abstract


Brazilian Journal of Biology, 2024, vol. 84, e253436 7/8

Providing inoculum for Didymella bryoniae studies

LEE, D.H., 1982. Morphological and cultural characters of Didymella 
bryoniae on seeds and culture media. Kor J Mycol, vol. 10, pp. 7-13.

LIU, S., SHI, Y., MIAO, H., WANG, M., LI, B., GU, X. and ZHANG, S., 
2017. Genetic analysis and qtl mapping of resistance to gummy 
stem blight in Cucumis sativus seedling stage. Plant Disease, 
vol. 101, no. 7, pp. 1-8. http://dx.doi.org/10.1094/PDIS-08-16-
1116-RE. PMid:30682960.

MAIA, F.G.M., ARMESTO, C., ZANCAN, W.L.A., MAIA, J.B. and DE 
ABREU, M.S., 2011. Efeito da temperatura no crescimento 
micelial, produção e germinação de conídios de Colletotrichum 
spp. isolados de mangueira com sintomas de antracnose. 
Bioscience Journal, vol. 27, no. 2, pp. 205-210.

MAO, X., WU, Z., BI, C., WANG, J., ZHAO, F., GAO, J., HOU, Y. and 
ZHOU, M., 2020. Molecular and biochemical characterization of 
pydiflumetofen-resistant mutants of Didymella bryoniae. Journal 
of Agricultural and Food Chemistry, vol. 68, no. 34, pp. 9120-9130. 
http://dx.doi.org/10.1021/acs.jafc.0c03690. PMid:32806116.

MERYMAN, H.T., 1966. Cryobiology. London and New York: 
Academic Press.

NGA, N.T.T., GIAU, N.T., LONG, N.T., LÜBECK, M., SHETTY, N.P., DE 
NEERGAARD, E., THUY, T.T.T., KIM, P.V. and JØRGENSEN, H.J.L., 
2010. Rhizobacterially induced protection of watermelon 
against Didymella bryoniae. Journal of Applied Microbiology, 
vol. 109, no. 2, pp. 567-582. http://dx.doi.org/10.1111/j.1365-
2672.2010.04685.x. PMid:20163499.

PULZ, P. and MASSOLA JR, N.S., 2009. Effect of culture media and 
physical factors on growth and sporulation of Alternaria dauci 
and A. solani. Summa Phytopathologica, vol. 35, no. 2, pp. 121-
126. http://dx.doi.org/10.1590/S0100-54052009000200007.

R DEVELOPMENT CORE TEAM, 2018. R: a language and environment 
for statistical computing, Vienna, Austria: R Foundation for 
Statistical Computing.

SAKR, N., 2019. Long term storage for five important cereal 
phytopathogenic species. Pakistan Journal of Phytopathology, 
vol. 31, no. 2, pp. 155-162.

SEPÚLVEDA, L., VÁSQUEZ, L.E., PANIAGUA, C.I., ECHEVERRY, D., 
HERNÁNDEZ, C.A., RODRÍGUEZ, E., RESTREPO, L.F. and ARANGO, 
R., 2009. The presence and spectrum of light influences the in 
vitro conidia production of Mycosphaerella fijiensis causal agent 
of black sigatoka. Australasian Plant Pathology, vol. 38, no. 5, 
pp. 514-517. http://dx.doi.org/10.1071/AP09036.

SKARSHAUG, A.J., 1981. Centrum development in Didymella bryoniae. 
American Journal of Botany, vol. 68, no. 8, pp. 1096-1103. http://
dx.doi.org/10.1002/j.1537-2197.1981.tb06393.x.

SOMAI, B.M., KEINATH, A.P. and DEAN, R.A., 2002. Development 
of PCR-ELISA for detection and differentiation of Didymella 
bryoniae from related Phoma species. Plant Disease, vol. 86, no. 
7, pp. 710-716. http://dx.doi.org/10.1094/PDIS.2002.86.7.710. 
PMid:30818565.

TORTORA, G.J., FUNKE, B.R. and CASE, C.L., 2011. Microbiologia. 10. 
ed. Porto Alegre: Artmed, pp. 964.

TSAY, J.G., TZEN, S.L. and TUNG, B.K., 1990. Enhancement of 
sporulation of Didymella bryoniae by near-ultraviolet irradiation. 
Plant Protection Bulletin, vol. 32, pp. 229-232.

TSUTSUMI, C.Y. and SILVA, N., 2004. Screening of melon populations 
for resistance to Didymella bryoniae in greenhouse and plastic 
tunnel conditions. Brazilian Archives of Biology and Technology, 
vol. 47, no. 2, pp. 171-177. http://dx.doi.org/10.1590/S1516-
89132004000200002.

BHAT, Z., DAR, G., BHAT, M. and ANHANGER, M., 2009. Effect of 
Media, Temperature and pH on growth and fructification of 
Didymella bryoniae (Auresw.) Rehm. causing blight in ridge 
gourd. Applied Biological Research, vol. 11, no. 5, pp. 70-72.

BRAGA, G.U.L., RANGEL, D.E.N., FERNANDES, É.K.K., FLINT, S.D. and 
ROBERTS, D.W., 2015. Molecular and physiological effects of 
environmental UV radiation on fungal conidia. Current Genetics, 
vol. 61, no. 3, pp. 405-425. http://dx.doi.org/10.1007/s00294-
015-0483-0. PMid:25824285.

CHAMBERLAIN, M. and INGRAM, D.S., 1997. The balance and 
interplay between asexual and sexual reproduction in fungi. 
Advances in Botanical Research, vol. 24, pp. 71-87. http://dx.doi.
org/10.1016/S0065-2296(08)60071-3.

CHIU, W.F. and WALKER, J., 1949. Morphology and variability of 
the cucurbit black rot fungus. Journal of Agricultural Research, 
vol. 78, no. 5, pp. 81-102.

CHOI, I.Y., CHOI, J.N., CHOI, D.C., SHARMA, P.K. and LEE, W.H., 2010. 
Identification and characterization of the causal organism 
of gummy stem blight in the muskmelon (Cucumis melo 
L.). Mycobiology, vol. 38, no. 3, pp. 166-170. http://dx.doi.
org/10.4489/MYCO.2010.38.3.166. PMid:23956648.

CORROCHANO, L.M., 2007. Fungal photoreceptors: sensory 
molecules for fungal development and behaviour. Photochemical 
& Photobiological Sciences, vol. 6, no. 7, pp. 725-736. http://
dx.doi.org/10.1039/b702155k. PMid:17609765.

GRUBE, M., FÜRNKRANZ, M., ZITZENBACHER, S., HUSS, H. and 
BERG, G., 2011. Emerging multi-pathogen disease caused by 
Didymella bryoniae and pathogenic bacteria on Styrian oil 
pumpkin. European Journal of Plant Pathology, vol. 131, no. 3, 
pp. 539-548. http://dx.doi.org/10.1007/s10658-011-9829-8.

GUSMINI, G., ELLINGTON, T.L. and WEHNER, T.C., 2003. Mass 
production of gummy stem blight spores for resistance screening. 
Report - Cucurbit Genetics Cooperative, vol. 26, pp. 26-30.

HASSAN, M.Z., ROBIN, A.H.K., RAHIM, M.A., NATARAJAN, S., KIM, 
H.T., PARK, J.I. and NOU, I.S., 2018. Screening of melon genotypes 
identifies gummy stem blight resistance associated with Gsb1 
resistant loci. Journal of Plant Biotechnology, vol. 45, no. 3, pp. 
217-227. http://dx.doi.org/10.5010/JPB.2018.45.3.217.

HAWKSWORTH, D.L. and COLWELL, R.R., 1992. Microbial diversity: 
biodiversity amongst microorganisms and its relevance. 
Biodiversity and Conservation, vol. 1, no. 4, pp. 221-226. http://
dx.doi.org/10.1007/BF00693760.

KEINATH, A.P., FARNHAM, M.W. and ZITTER, T.A., 1995. 
Morphological, pathological, and genetic differentiation of 
Didymella bryoniae and Phoma spp. isolated from cucurbits. 
Phytopathology, vol. 85, no. 3, pp. 364-369. http://dx.doi.
org/10.1094/Phyto-85-364.

KWON, M.K., HONG, J.R., SUN, K.Y., CHO, B. and KIM, K.C., 
1997. Standardization of a mass-production technique for 
pycnidiospores of Didymella bryoniae, gummy stem blight fungus 
of cucurbits. Korean J. Plant Pathol, vol. 13, no. 2, pp. 105-112.

LEACH, C.M., 1962. The quantitative and qualitative relationship of 
ultraviolet and visible radiation to the induction of reproduction 
in Ascochyta pisi. Canadian Journal of Botany, vol. 40, no. 12, pp. 
1577-1602. http://dx.doi.org/10.1139/b62-154.

LEÃO, E.U., SANTOS, G.R., SARMENTO, R.A., REIS, M.R. and CHAGAS 
JUNIOR, A.F., 2012. Crescimento micelial e produção de conídios 
de Ascochyta cucumis em diferentes meios de cultura e regimes 
de luz. Bioscience Journal, vol. 28, no. 2, pp. 325-331.

https://doi.org/10.1094/PDIS-08-16-1116-RE
https://doi.org/10.1094/PDIS-08-16-1116-RE
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=30682960&dopt=Abstract
https://doi.org/10.1021/acs.jafc.0c03690
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=32806116&dopt=Abstract
https://doi.org/10.1111/j.1365-2672.2010.04685.x
https://doi.org/10.1111/j.1365-2672.2010.04685.x
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=20163499&dopt=Abstract
https://doi.org/10.1590/S0100-54052009000200007
https://doi.org/10.1071/AP09036
https://doi.org/10.1002/j.1537-2197.1981.tb06393.x
https://doi.org/10.1002/j.1537-2197.1981.tb06393.x
https://doi.org/10.1094/PDIS.2002.86.7.710
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=30818565&dopt=Abstract
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=30818565&dopt=Abstract
https://doi.org/10.1590/S1516-89132004000200002
https://doi.org/10.1590/S1516-89132004000200002
https://doi.org/10.1007/s00294-015-0483-0
https://doi.org/10.1007/s00294-015-0483-0
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=25824285&dopt=Abstract
https://doi.org/10.1016/S0065-2296(08)60071-3
https://doi.org/10.1016/S0065-2296(08)60071-3
https://doi.org/10.4489/MYCO.2010.38.3.166
https://doi.org/10.4489/MYCO.2010.38.3.166
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=23956648&dopt=Abstract
https://doi.org/10.1039/b702155k
https://doi.org/10.1039/b702155k
https://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=17609765&dopt=Abstract
https://doi.org/10.1007/s10658-011-9829-8
https://doi.org/10.5010/JPB.2018.45.3.217
https://doi.org/10.1007/BF00693760
https://doi.org/10.1007/BF00693760
https://doi.org/10.1094/Phyto-85-364
https://doi.org/10.1094/Phyto-85-364
https://doi.org/10.1139/b62-154


Brazilian Journal of Biology, 2024, vol. 84, e2534368/8

Virtuoso, M.C.S. et al.

TUKEY, J. W., 1953. The problem of multiple comparisons. New York: 
Chapman and Hall. Unpublished memorandum in private 
circulation.

WIANT, J.S., 1945. Mycosphaerella black rot of cucurbits. Journal 
of Agricultural Research, vol. 71, no. 5, pp. 193-214.

WOLUKAU, J.N., ZHOU, X.H., LI, Y., ZHANG, Y-B.. and CHEN, J.-F., 
2007. Resistance to gummy stem blight in melon (Cucumis 
melo L.) germplasm and inheritance of resistance from plant 

introductions 157076, 420145, and 323498. HortScience, vol. 42, 
no. 2, pp. 215-221. http://dx.doi.org/10.21273/HORTSCI.42.2.215.

ZHANG, N., XU, B.H., BI, Y.F., LOU, Q.F., CHEN, J.F., QIAN, C.T., ZHANG, 
Y.B. and YI, H.P., 2017. Development of a muskmelon cultivar 
with improved resistance to gummy stem blight and desired 
agronomic traits using gene pyramiding. Journal of Genetics 

and Plant Breeding, vol. 53, no. 1, pp. 23-29. http://dx.doi.
org/10.17221/84/2016-CJGPB.

https://doi.org/10.21273/HORTSCI.42.2.215
https://doi.org/10.17221/84/2016-CJGPB
https://doi.org/10.17221/84/2016-CJGPB