24th Int. Symp. “Animal Science Days”, Ptuj, Slovenia, Sept. 21st−23rd, 2016.
Acta argiculturae Slovenica, Supplement 5, 143–147, Ljubljana 2016
COBISS: 1.08
Agris category code: L73
 
MICROSPORIDIAN NOSEMA SPP. AS A MODEL GASTROINTES-
TINAL MICROORGANISM OF CARNIOLAN HONEY BEE (APIS 
MELLIFERA CARNICA, POLLMAN, 1879): ASPECTS OF SPORE 
COUNTING
Ilja Gasan OSOJNIK ČRNIVEC 1, 2
Microsporidian Nosema spp. as a model gastrointestinal microorganism of Carniolan honey bee (Apis mellifera carnica, Pollman, 
1879): Aspects of spore counting
 
1 Agricultural Institute of Slovenia, Animal Production Department, Hacquetova 17, SI-1000 Ljubljana, Slovenia
2 New address: University of Ljubljana, Biotechnical Faculty, Department of Animal Science, Groblje 3, SI-1230 Ljubljana, Slovenia, e-mail: gasan.osojnik@bf.uni-lj.si
ABSTRACT
At high invasion levels, nosemosis can act as an underlying cause of colony collapse disorder, especially in cases 
of simultaneous invasion of other parasites or/and in combination with virus infections. Rapid quantitative methods 
for Nosema spp. spore detection are therefore required for various research and diagnostic needs. In this study, the use 
of haemocytometer (standard method) and Coulter counter is compared. All work was performed with late summer 
forager bees of Carniolan honey bee subspecies, prepared as isolates and homogenates of the posterior section of the 
worker bee’s intestine. It can be concluded that the Coulter counter provides greater sample dilution flexibility at suf-
ficient repeatability (RSD 0.01–0.1) in the cases of: (i) low concentrations of spores, as well as (ii) samples that required 
high dilutions (c ≥ 107 spores ml–1). However, Coulter counter use required additional data processing for obtaining 
precise concentration estimates at ~ 3 µm mean spore size. Nevertheless, the uncorrected, as-measured values provided 
concentration ranges which were found to be suitable for general diagnostic purposes.
Key words: bees, Carniolan honey bee, microbiology, microorganisms, cell counting, haemocytometer, Coulter 
counter
1 INTRODUCTION
Nosema disease, or nosemosis of honey bees is 
presently known to be caused by two species of micro-
sporidian parasites, Nosema apis (Zander, 1909) and 
Nosema ceranae (Fries et al., 1996). Spores of the two 
Nosema species have similar ovoid morphologies. Spores 
of N. ceranae are slightly smaller, reportedly measuring 
3.3–5.5 µm length and 2.3–3.0 µm width, whereas N. apis 
spore ranges are 4–6 µm and 2–4 µm, respectively (Fries 
et al., 1996; Higes et al., 2010). Both species invade the 
epithelial cells of ventriculus (midgut) and have similar 
life cycles, resulting in release of large number of spores 
and in severe cases, in consequential death of bees due to 
destruction of the intestine wall. At high invasion levels, 
nosemosis can act as an underlying cause of colony col-
lapse disorder, especially in cases of simultaneous inva-
sion of other parasites and/or in combination with virus 
infections (Bromenshenk et al., 2010).
Due to continuous honey bee colony losses, stand-
ing requirements for data collection on parasite pathol-
ogy, omnipresence within the honey bee population and 
simplicity of observation, the microsporidian Nosema 
spp. was selected as a model gastrointestinal microorgan-
ism for a study on spore counting aspects, which can be 
extended to cell counting applications.
Routinely, a haemocytometer is used for the quanti-
tative particle analysis of bee gut contents, in particularly 
for assessment or spores of Nosema spp. Simultaneous 
analyses of other microorganisms residing in the bee gut 
increase the counting time and typically require prelimi-
nary staining procedures. In this study, an insight in re-
liability of a traditional haemocytometer counting tech-
nique for Nosema spp. spore assessment is provided and 
the method is compared to the performance of a portable 
Acta agriculturae Slovenica, Supplement 5 – 2016144
I. G. OSOJNIK ČRNIVEC
suming spherical morphologies. The procedure is auto-
mated and typical sample handling time ranged from 1 
to 3 minutes. For spore counts, sensors with 40 µm ap-
erture were used. Prior use, the apparatus was assessed 
for reliability with a reference suspension of polystyrene 
beads (d = 15 µm, cp = 2 × 10
5 beads ml–1) using 40 and 
60 µm sensors (sensor measuring ranges within 3–17 and 
6–36  µm, respectively). Reference measurements con-
sistently showed high repeatability of results with both 
sensor types (relative standard deviation, RSD  <  0.06, 
c p  =  2.3  ×105  beads  ml−1). Cell counts in the desired 
uniform particle size range were obtained with Scepter 
Software 2.1 (Merck) cellular analysis platform. In order 
to extrapolate particle size concentration and distribu-
tion below the detection range of the 40 µm sensor, peak 
fitting (Gaussian amplitude / peak function) was per-
formed with Origin 8.1 (OriginLab Corporation) data 
analysis software.
In parallel to the novel automated counting meth-
od, counting was performed using a Bürker chamber 
(12 × 12 fields) under Leica DM 2500 light microscope 
at 400 × magnification. Typical sample handling time for 
this method ranged from 10 to 20 minutes.
3 RESULTS AND DISCUSSION
Initially, the standardised method was employed 
for spore counting for an array of samples, which were 
exhibiting a wide range of Nosema spp. levels of infec-
tion (from 105–107  spores  ml–1), as shown in Table 1. 
Preliminary tests showed high variability (P  <  0.001, 
Coulter cell counter for examination of a complex sam-
pling matrix of bee gut homogenate.
2 MATERIAL AND METHODS
All work was performed with the subspecies Car-
niolan honey bee (Apis mellifera carnica, Pollman, 
1879). Forager bees of sufficient quantity (approximately 
100  bees/hive) were sampled during July and August 
2015 from hives located at various field stations operat-
ing within the Slovenian national bee monitoring net-
work. Bees were sampled at the hive entrance, in order 
to avoid underestimation of spore count via sampling of 
recently-hatched bees which are spore-free.
Sample preparation (isolation and homogenisation 
of the posterior section of the worker bee’s intestne) and 
haemocytometer counting were performed following 
the standard methods, described by Fries et al. (2013) 
and Human et al. (2013), respectively. For all samples 
analysed, phosphate-buffer saline was used instead of DI 
water to ensure conductivity of the samples, which was 
required for particle size determination by means of the 
Counter principle.
A portable Coulter counter was used to count sam-
ples (Merck, model Scepter 2.0 Cell counter). The basic 
operational principle of the device consists of pumping 
a conductive suspension (sample) through a microchan-
nel and determining the particle size of passing solids 
from measured changes in impedance, which are directly 
proportional to the volume of the particle traversing 
the orifice. The particle diameter is then calculated as-
Replicate N° Hive I Hive II Hive III Hive IV Hive V Hive VI Hive VII
1 0.45 1.7 3.5 4.3 11.3 20.8 27.8
2 0.5 1.8 3.1 3.8 10.8 20.8 28.4
3 0.7 1.7 3.6 5.7 10.7 19.25 27.2
4 0.6 1.5 3.7 5.4 10.6 19.55 27.9
5 0.65 1.8 3.6 3.9 9.2 20.3 27.1
6 0.6 2.1 3.1 4.1 9.05 20.1 27.3
7 0.6 2.1 2.9 5.1 10.1 19.9 27.1
8 0.45 2.3 4.5 4.0 10.5 19.1 27.5
9 0.55 1.9 3.7 3.7 9.7 20.0 27.1
10 0.7 1.4 3.6 5.2 10.2 20.1 27.3
Average ± SD 0.58 ± 0.09 1.82 ± 0.28 3.49 ± 0.44 4.50 ± 0.75 10.22 ± 0.72 19.99 ± 0.57 27.45 ± 0.44
RSD 0.16 0.15 0.13 0.17 0.07 0.03 0.02
units of concentration: × 106 spores ml−1
Table 1: Spore concentration, average ± standard deviation and haemocytometer counting repeatability (RSD) for seven hives with 
different Nosema spp. levels of infection
Acta agriculturae Slovenica, Supplement 5 – 2016 145
MICROSPORIDIAN NOSEMA SPP. AS A MODEL ... (APIS MELLIFERA CARNICA, POLLMAN, 1879): ASPECTS OF SPORE COUNTING
et al., 2015; Emsen et al., 2016) and monitoring stud-
ies report N. ceranae domination in population share, 
as well as in prevalence. As the need of differentiation 
amongst the two Nosema species has decreased in im-
portance for general diagnostic purposes, spores in this 
study were regarded as one population with the Coulter 
counter device. Nevertheless, the counting method does 
allow for some basic recognition, taking in mind the 
particle diameters provided by the Coulter counter are 
represented as sphere diameters, whereas Nosema spores 
exhibit prolate ovoid morphologies. Assuming 50 % N. 
apis and 50 % N. ceranae population, prolate ovoids with 
3.3–6 µm in length and 2.3–4.0 µm in width would have 
been observed in the sample, corresponding to an meas-
ured average sphere diameter of 3.6 µm. However, as it 
is evident from Figure 1, the average sphere diameter 
has been extrapolated to fall below 3 µm (conforming to 
ovoid shapes with roughly 4 µm in length and 2.5 µm in 
width), indicating an expected dominance of N. ceranae 
spores and simultaneously confirming the coexistence of 
N. apis spores in the examined samples.
The employed portable Coulter counter is capable of 
detection of particles, which are larger than 3 µm and at 
these limitations the device operates within the 5 × 104–
1.5 × 106 particle ml–1 concentration range. Using the ap-
proach presented in Figure 1, it is possible to extrapolate 
the measured values to obtain total spore counts and 
dimensions. In comparison to counts obtained with the 
standard spore counting procedure, the adjusted values 
were analogous (90.4 % match).
Furthermore, uncorrected, as-measured values 
( c 1–3 = 1.22 × 107 spore ml–1) accounted for approximate-
0.2–0.5  RSD) of spore counts from bees sampled from 
the same hive for separately prepared and thoroughly ho-
mogenized suspensions (n = 20 / 3 suspensions / 4 hives). 
Therefore in order to increase the level of repeatability, all 
subsequent analyses were performed with the same pri-
mary material per hive. Furthermore, ten replicates of the 
same sample were evaluated by counting either twelve 
or five fields in the counting chamber and the results 
were found to be comparable (an average count ratio for 
12/5 fields of 0.99/1 was obtained). From there on, five 
fields were used for counting (1/1; 1/12; 12/1; 12/12; 6/6), 
at it is mostly done in internal routine counting appli-
cations. Using this approach it is evident that at lower 
concentrations (up to 4.5  ×  106  spores  ml–1), where 
1–20  spores can be counted for each field, the coeffi-
cient of variation between replicates was relatively high 
(Table 1). To increase the repeatability of these results, 
more fields could have been counted (consequently in-
creasing the time of analysis). At higher concentrations 
(20–140 spores per field), repeatability was high and the 
coefficient of variation was well below 10 %.
For the purpose of examination of the counting 
method based on the Coulter principle, we selected a 
sample exhibiting high Nosema spp. level of infection. 
For each sample, two series of triplicates were measured 
and respective particle-size distributions were extrapo-
lated below the lower limit of measurement to the full ex-
pected diameter range (as shown in Figure 1 for the case 
of a 100 × diluted sample). Within samples, good repeat-
ability of measurements, as well as a good fit to normal 
distribution were observed.
In the recent years, several researchers (e.g. Csáki 
2.5 3.0 3.5 4.0 4.5
0
300
600
900
1200
0
300
600
900
1200
0
300
600
900
1200
2.5 3.0 3.5 4.0 4.5
Fd = 100
c3= 2.53 × 10
7 spore ml-1  
Diameter (µm)
 triplicate 3
Fd = 100
c2= 2.46 × 10
7 spore ml-1
Co
un
t
 triplicate 2
Fd = 100
c1= 2.46 × 10
7 spore ml-1
R2= 96.5 %
R2= 96.8 %
 
 triplicate 1
R2= 96.6 %
Figure 1: Particle diameter and count in 100 × diluted sample of bee gut homogenates. Difference between triplicates not statistically 
significant (P > 0.05).
Acta agriculturae Slovenica, Supplement 5 – 2016146
I. G. OSOJNIK ČRNIVEC
ly two fold lower concentrations, yet they remained in 
the same order of magnitude in comparison to the refer-
ence value which was determined by the standard count-
ing method.
As both counting techniques require sample dilu-
tion at high spore concentration, a dilution series was 
prepared to study possible effects. The haemocytomet-
ric spore count of the undiluted sample was set as the 
reference value (Figure  2, denoted as dashed line). For 
the case of undiluted sample, high repeatability of counts 
was obtained at  >  100  spores for each counting field. 
However, analyses of larger sets of samples having such 
a concentration range require a lot of time and focused 
concentration of the microscope operator. It is therefore 
not uncommon to count Nosema spp. spores in 10 × di-
luted samples, where reliable counts can be achieved, as 
Figure 2 shows.
At higher dilutions (100  and  1000  ×) beyond the 
recommended spore concentration of 5–50  spores per 
field (Human et al. 2013), the spore numbers became in-
creasingly overestimated (up to 180 %). In the case of the 
standard method, increasing the dilution did not affect 
the coefficient of variation (in order of dilution: 13  %, 
9 %, and 7 %).
Using the Coulter counter adjusted values at 10  × 
sample dilution (operating slightly above the recom-
mended concentration) 30  % underestimation of the 
spore concentration was observed. In contrast to stand-
ard counting method, Coulter counter provided relevant 
values (up to 93 % of the reference value) in subsequent 
dilutions. In this case, the coefficient of variation was in-
creased from 1 % at 10 × dilution to 10 % at 1000 × dilu-
tion.
Similarly to previous observations, uncorrected val-
ues corresponded to 40–77 % (2.5–1.3 fold) of the adjust-
ed concentration at 10–1000 × dilution, respectively. This 
apparent discrepancy can be explained by the fact that 
as the number of the spores in the suspension decreases 
due to dilution, the size fraction of the spores which is 
numerically most represented in the initial (undiluted) 
population, gains an even greater effect on the overall 
population estimate. Furthermore, adjusted and unad-
justed values exhibited the same coefficients of variation, 
indicating that the extrapolation has been performed 
correctly as it preserves the initial characteristics of the 
measurements within the expanded set of data.
4 CONCLUSIONS
Nosema spp. was selected as a model gastrointesti-
nal microorganism for a study on spore counting aspects, 
which can be extended to cell counting applications. Two 
methods, (i) standard haemocytometer counting tech-
nique and (ii) the use of a Coulter counter are compared.
It can be concluded, that the Coulter counter pro-
vides greater dilution flexibility and exhibited sufficient 
accompanying repeatability (RSD 0.01–0.1) for the anal-
ysis of: (i) spores at low concentrations, or (ii) samples at 
high dilutions.
Counting spores at low and medium concentrations 
(6 × 105–4 × 106 spore ml–1) using the standard method 
resulted in borderline repeatability (RSD up to 0.17), 
indicating that prolonged sample observation was re-
quired, as an increased number of fields would have had 
of been visually examined.
0 10 100 1000
0
1
2
3
4
5
 
Co
nc
en
tra
tio
n 
(×
 1
07
 s
po
re
s 
m
l-1
)
Dilution factor
 Standard method
 Corrected Coulter counter
 Coulter counter
re
fe
re
nc
e
   
   
  v
al
ue
Figure 2: Spore concentration average at different sample dilutions for each counting method (bars denote standard deviation)
Acta agriculturae Slovenica, Supplement 5 – 2016 147
MICROSPORIDIAN NOSEMA SPP. AS A MODEL ... (APIS MELLIFERA CARNICA, POLLMAN, 1879): ASPECTS OF SPORE COUNTING
High sample dilutions may be required, e.g. when 
analysing concentrations ≥ 107  spores  ml–1. At higher 
concentrations (3  ×  107  spores  ml–1), the repeatability 
of the traditional technique was high (RSD < 0.05), and 
the sample handling time was longer as a result of higher 
spore counts. In the case of unsuitably high dilutions, the 
measured concentrations were imprecise.
The downside of using Coulter counters is that ad-
ditional data processing techniques may be required. It 
is furthermore important to note that the entire spore 
concentration range, and simultaneous presence of other 
microorganisms (e.g. yeasts with typical dp  =  3–4  μm) 
were not evaluated in this study and that these effects on 
Nosema spore counting should be considered further. 
Nevertheless, in comparison to reference value, similar 
spore concentrations were observed when using adjusted 
Coulter counter counts. At 100 and 1000 × dilution, ad-
justed values consistently corresponded to roughly 90 % 
of the set reference value, showing that this approach can 
be used for obtaining precise total counts. To allow for 
time efficient analyses, such devices should allow for the 
integration of advanced data processing techniques.
Uncorrected values show two to three fold lower 
concentrations, yet they remain in the same concen-
tration range than the reference value (e.g. 107 for the 
presented case) and could therefore be used for routine 
diagnostic purposes, where the information of the exact 
concentration is not required.
5 ACKNOWLEDGEMENTS
The author gratefully acknowledges various techni-
cal help, sample selection assistance and diligent work 
with biological material from David Kozamernik, Mitja 
Nakrst and Mateja Soklič (Agricultural institute of Slo-
venia) as well as from high school students Teja Rus and 
Anja Seliškar (Biotechnical Educational Centre Ljublja-
na).
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