QUALITY ASSESSMENT OF HONEY EXTRACTED USING TRADITIONAL METHODS FROM SOME HONEY BEARING COMMUNITIES OF KADUNA STATE
QUALITY ASSESSMENT OF HONEY EXTRACTED USING TRADITIONAL METHODS
FROM SOME HONEY BEARING COMMUNITIES OF KADUNA STATE
ABSTRACT
Twelve commercial honey samples obtained using five different
traditional methods of honey extraction, from some honey bearing communities of
Kaduna State Nigeria, were analysed using laboratory analytical procedures and
ANOVA statistical tool to determine the effects of traditional methods of honey
extraction on the products quality parameters. The parameters determined
alongside their range for the honey samples, included moisture content (15.50 –
22.00%), ash content (0.50 – 0.85%), pH (3.44 – 4.16), total acidity (0.12 –
0.37%), reducing sugar (50.08 – 54.20%), sucrose (26.61 – 28.80%), density
(1322.35 – 1382.16g/L) and water insoluble content (1.30 – 1.70%) were
obtained. For the microbiological characteristics; total bacteria plate count
(1.7 x 102 – 9.8 x 103 cfu/g), total coliform count (1.3
x 102 – 7.7 x 103 cfu/g) mould count (2.0 x 101
– 1.5 x 103 cfu/g), while both yeast and E. coli were not detected
in any of the samples. The ANOVA result revealed there were significant
differences both within the methods of extraction and the percentage mean
values of the quality parameters of commercial honey samples extracted and marketed
in different retail outlets in Kaduna State. Although the honey samples had
good shelf life and fairly – good physical properties, they, however, contained
high water insoluble contaminants such as honey-wax; had been adulterated with other substances
like sugarcane sugar or corn syrup; and were also highly susceptible to attack
by pathogenic micro organisms and fermentation. To address these challenges, it
was recommended that commercial bee farmers and honey producers in the state be
mobilized into forming a strong cooperative society to easily access cooperate
supports via enlightenment; retraining, capital (grants or loans) support from
the Nigerian Agriculture, Cooperative and Rural Development Bank (NACRDB) to
acquire standard extraction equipment and facilities, and the establishment of
honey monitoring and quality assessment centres by the state government, among
others.
CHAPTER 1
INTRODUCTION
1.1
BACKGROUND
OF THE STUDY
It has been reported that honey stored, processed
and sealed by honey bees in the cells of their comb is always of good quality,
but the different management methods and techniques of honey harvesting,
extraction, and storage greatly influence the quality and marketing of the product
(Mutsaers, 1991). Hence, _honey as the
most important product of beekeeping both from a quantitative and an economic
points of view_has been defined as the natural sweet substance produced by honey bees from nectar of plants
(nectar honey), or from secretions of living parts of plants, or excretions of
plant sucking insects on the living parts of plants (honeydew honey) which
honey bees collect, transform by combining with specific substances of their
own, deposit, dehydrate, store and leave in the honey comb to ripen and mature
(Bogdanov, et al., 2001). Thus, the importance and uses of honey is
parallel to the history of man and in virtually every culture. Evidence can be
found of some of its enormous uses as: an ancient valuable food and food
derivative; as a medicinal aid for fighting infections (as an ointment for
rashes, wounds and burns, and to help soothe sore throats) and diseases (as a
comprehensive treatment of diabetic ulcers); and as a symbol employed in
religious, magic and therapeutic ceremonies (Jennifer, 2007; Mark, 2008, Molan,
1999).
Consequently, owing to the vast applications and
benefits derivable from honey, the current total annual world production of the
product (honey) stands at, 1,134,000 tonnes; with the exception of some
counties, like Nigeria_whose production level of honey is predominantly still
on a subsistence and seasonally - small_scale commercial classification (Honey Travelers,
2011), and whose bulk of honey producers widely adopt the traditional methods
of honey extraction. Mutsaers (1991), therefore, further added that some of
these traditional methods of honey extraction can easily damage the quality of
the product when poorly applied. For instance, he stated that methods which use
heat, fire or boiling of honey will produce honey that is dark, dirty and has a
reduced medicinal and health values. Thus, he concluded by quoting; “After having
gone through so much care and trouble to produce high quality honey, it is a
pity to spoil it by poor extraction methods”.
In addition, Honey Travelers (2011) remarked that
unheated “raw” honey contains all the vital ingredients that give it its
healthful properties and wonderful aroma; unfortunately, most commercial honey
one sees in supermarkets and retail outlets in Kaduna State is not raw honey,
this mass – produced honey is often heated by some traditional extraction
methods, such as solar melting, to temperatures far above the normal
temperatures of the bee hive (350C); in order to make the product
(honey) easier to extract from the honey comb, to filter it and to package it
among other reasons. This extraction method, thus changes honey’s essential
composition and degrades its quality by partially destroying honey’s beneficial
enzymes and boils off volatile compounds (vitamins such as Riboflavin, Niacin and Pantothenic) that account for the
unique delicate flora aroma of the honey (Gheldof, et al., 2002). Furthermore,
although, it is widely believed that honey, in its natural state in the
honey comb, cannot spoil nor borne disease – causing – organisms, but some
traditional methods of honey extraction, such as hand – squeezing and sieving, easily expose the product to
direct bacteria infestation mainly through dirty hands and unhygienic
processing vicinity. Thus, increasing the risk of possible health hazards, such
as Botulism and Honey intoxication, to its consumers (Food and Drug
Administration, FDA, 2012 and The National Honey Board, 2012).
Unarguably, wholesomeness of food products that guarantee
the safety of the consumers is the most important attribute of food quality
(Oyinlola, 2004). Hence, in order to have a comprehensive quality assessment of
any food product, it is of great necessity that the areas of purity, safety,
economics, taste, appearance, prevailing legislative regulation, and consumer
expectations are adequately examined (Ojeme, 1990). Although most marketers and
consumers of honey in Kaduna state had been using some traditional physical
techniques; such as match-stick-test to estimate the degree of moisture of
honey, pouring honey into a transparent glass cup of cold water to determine
its viscosity, putting drop of honey on the floor whether ants will approach it
or not, to estimate its sugars level; to assess the quality of honey. All these
techniques are highly questionable and unreliable. Unfortunately, not all
marketers and consumers of these traditionally extracted honey can easily and
quickly ascertain some of these intrinsic quality parameters of the product.
Therefore, this project intends to identify and analyze the various traditional
methods of honey extraction _ using some honey bearing communities of Kaduna
state, Nigeria, as case study _ and any adverse effects such methods may have
on the quality parameters of the product.
1.2 STATEMENT
OF THE PROBLEM
Some
of the most prominent problems associated with the need for the study are as
follow:
1.2.1 Excessive moisture content of extracted
honey; thereby enhancing rapid fermentation of the product.
1.2.2 Thinning of honey viscosity via the
application of excessive heat, fire or boiling to ease extraction and packaging
processes; thereby producing honey that is dark, dirty and has a reduced
medicinal and health values.
1.2.3 Lack of personal hygiene (poor hand washing),
and carrying out honey extraction in unhygienic environments; thereby making
the product easily susceptible to germs infestation.
1.2.4 Use of unsuitable containers or extraction
equipment that have not been properly sterilized or not compatible with the
acidic nature of honey; thereby giving the product unpleasant odour and impure
texture.
1.2.5 Adulteration of honey by the addition of corn
or sugar-cane syrups, or any other contaminants to augment the quantity of the
extracted product for much profitability; thereby posing grave danger to the
health of ignorant consumers.
1.3 AIM
AND OBJECTIVES OF THE STUDY
1.3.1 AIM OF THE STUDY
The study aims at carrying out a quality assessment
of honey samples extracted, using traditional methods, from some honey bearing
communities of Kaduna state, Nigeria.
1.3.2 OBJECTIVES OF THE STUDY
The study hopes to achieve the following objectives;
(i)
Collect samples of honey extracted using
different traditional methods:
(ii)
Carryout laboratory analysis on the
samples collected;
(iii)
Assess the results obtained and compare
them with the quality template of honey, as laid down by the Nigerian
Industrial Standard (NIS 473:2003).
(iv)
Ascertain its suitability for both human
and industrial consumption
(v)
Make feasible recommendations on the results
analysed, where necessary.
1.4 SIGNIFICANCE
OF THE STUDY
The study, when concluded and all its
recommendations carefully implemented, will assist in achieving the following:
(i)
Reveal the level of conformity of the
quality of honey extracted using traditional methods and equipment with the
standard laid down by the Nigerian Industrial Standard (NIS 473:2003)
(ii)
Ascertain doubts about the hygienic
conditions of honey – extraction – containers and other processing equipment,
so as to determine whether or not the product is safe for human consumption.
(iii)
Honey samples(s) whose overall quality
parameters determined successfully meet up with the range recommended by the
Nigerian Industrial Standard (NIS 473:2003), can be safely used as sugar
substitute in confectioneries, and as health enhancer in medicine.
(iv)
Adequate information about the overall
quality parameters of honey samples, at public domain, will enhance the
marketability of the product, and also add value to the local honey businesses.
1.5 SCOPE
OF THE STUDY
The
study focuses on honey extracted using traditional methods Floating, Honey
pressing, Hand squeezing, Solar melting (heating), and Sieving methods obtained
from Ankwa, Doka, Giwa, Kafancha, Katari, Kukui, Mando and Sabon gari honey-bearing-
communities of Kaduna State, Nigeria. The laboratory analysis of the quality
parameters; the moisture content, ash content, total acidity (lactic acid), pH,
sucrose content, reducing sugar level, water insoluble content, density, and microbiological
characteristics of the samples collected will be carried out at the Departments
of Agricultural Engineering; Food Technology; and Applied science; all of
Kaduna Polytechnic. The result of the analysis will be compared with the
Nigerian Industrial Standard (NIS 473;2003) for honey and feasible
recommendations for further actions, presented.
CHAPTER
II
LITERATURE
REVIEW
2.0 HONEY EXTRACTION
Mustsaers (1991) defined honey
extraction as the central process in bee keeping of removing honey from honey
comb, so that it is isolated in pure liquid form. This invariably, implies that
whichever method of honey extraction that may be adopted by any honey producer be
it the traditional method or modern method the resulting product is expected to
be in a distinct and pure liquid form. Regretably, Mustsaers (1991) reported
that most traditional methods and equipment employed in honey extraction do not
concur with this definition: lack of personal hygiene (poor hand washing); use
of unsuitable containers (non food-graded) that have not been properly sterilized;
extraction of honey in the open/unhygienic environment; and eventual storing of
the product in poorly sealed containers, cause the product (honey) to become
easily adulterated and consequently, degenerated.
In view of the backlog of challenges posed by most
traditional methods of honey extraction; with respect to the overall quality
rating of the product, the centrifuge method was highlighted by Mustsaers
(1991) as the most modern and widely used method of honey extraction by many
large scale honey producers. In this method, as shown by Plate 1, the honey
comb (uncapped) is placed inside frames and arranged in an apparatus
(centrifuge extractor) consisting essentially of a compartment spun about a
central axis to separate the honey from other materials of different specific
gravities via the action and effect of a centrifugal force. This results in the
formation of different layers by the particles in a colloidal solution, after
which the honey, in liquid below the particles can be gently filtered-out. This
method is quick and more efficient.
Plate 1: Centrifuge method of honey extraction
2.1 TRADITIONAL
METHODS OF HONEY EXTRACTION
Honey extraction using traditional methods and
equipment varies across different geographical locations and societies. Where
as some societies view honey as a much revered, valuable and highly beneficial
commodity that requires the utmost care and attention during its extraction
processes, others see the product as a mere sweetener that does not deserve any
special treatment during its extraction. As such, the latter handles the
processes carelessly; thereby impacting negatively on the product’s overall
quality rating, (Surendra, 2008).
However, Adjare (1990) and Mustsaers (1991) both
presented a concise report on the most common traditional methods of honey
extraction, which are found in most geographical locations around the world.
They are as follow:
2.1.1 FLOATING METHOD: In this method, the
honey comb with capped honey (that is, honey comb filled with honey) is
uncapped with the aid of a slightly heated knife. The combs are later chopped
into pieces and put into an air – tight container(s) for about two days, to
settle down; otherwise exposure to damp air increases honey’s moisture content
(owing to honey’s hygroscopic nature) and the ease with which it ferments.
After the two days period of being allowed to settle down elapses, the wax
would have floated to the surface of the mixture leaving the honey below as
shown by Plate 2. The wax is then skimmed off while the honey is filtered out
via a clean cheese cloth or lace curtain material. The honey may be allowed to
settle down for an extra day in order to remove further any remaining foam and
wax particles.
Although a simple method, floating
has the following limitations:
·
It is time consuming.
·
The risk of honey being contaminated by
hands is high.
·
An already chopped comb can not be
returned to the beehive for re-use by the bees. This reduces productivity level
of the colony as more energy have to be subsequently spent on building another
honey comb by the bees.
Plate 2: Floating method of honey extraction
2.1.2 HONEY PRESSING METHOD: Here, the honey comb is first decapped and
chopped into smaller pieces in a plastic container, after which it is transferred
into a clean cloth or sack tightly wrapped_up or knotted at the opening, with
netting at the bottom, which fits in a double pot positioned under the honey
press. Thereafter, the filled sack is subjected to immense pressure by the
press which expels the honey out from the sack and then drip on to trays during
uncapping as shown in Plate 3. The scrap honey in the container (pot) is then
sieved. A number of honey pressing machines are available depending on the
desired capacity. They generally take the form of a simple hinged press or a press
with a spindle which is used to move one plate down on to the other to squeeze
the honey out from comb.
The major limitations associated
with the honey pressing method include:
·
Lost of the honey comb; meaning that the
colony has to build a new comb.
·
Low extraction efficiency and low work
rate; Ng’atiwa (1989) reported an extraction efficiency of about 58%, while Mutsaers
(1991) concluded that, whereas the honey press can be used for extracting small
quantity of honey
(2
kg/hr) a centrifuge is more efficient for quantities above 2kg/hr.
Plate
3: Honey pressing method of honey extraction
2.1.3 HAND – SQUEEZING METHOD:
This method of honey extraction is common
with bee farmers and few honey producers who desire to consume the
product themselves, or supply to consumers based on specific order. For
instance, in Milkwood Bay, Port Elizabeth, South Africa, (Tim, 2012) reported
that the locals, after collecting the honey combs from the hives, they cut the
honey comb off the top-bars, after which all the honey comb are crushed and
meshed in a plastic container as shown by Plate 4(a) & (b). For this
harvest, they placed a big sieve on top of a honey bucket with a gate on the
front, after which the crushed and meshed comb is poured or tipped into the
sieve alongside some older stuff from a previous harvest. To speed_up the
process, they will all squeeze the comb by grabbing great handfuls; this meant
they expelled the honey from the wax much quicker. At the end of this process,
about 5kg strained honey (from 3 combs, and about 0.5kg of bee wax in lumps)
are obtained. These entire processes result to pure, cold-pressed organic honey
that have got everything that was in the honey; pollen, propolis and lots more.
They get honey that is not heated in anyway during the process, which means
none of the delicate antibiotics and enzymes within the honey are destroyed.
Finally, they will pour all into a jar without further filtration.
Nonetheless,
honey extraction by hand squeezing method has the following limitations;
·
High level of pollen content in
extracted honey may pose an aesthetic concern in terms of marketability or long
term storage.
·
Unhygienic hands easily contaminate the
honey, and fermentation may occur after few days.
Plate 4 (a) & (b): Hand-squeezing method of
honey extraction
2.1.4 SOLAR MELTING METHOD: This method is also referred to as the
‘Heating’ method because it involves the application of heat energy in melting-
out honey from the honey comb. Unlike the crude means in which live embers are
placed on a pile of capped honeycombs to extract the honey, this method adopts
the use of a relatively safe solar radiation of the sun. In this method, the
capped honey comb is first decapped and chopped into smaller pieces in a
plastic container, after which it is transferred into a wide woven basket made
of palm leaves. The woven basket is placed on top of a plastic basin into which
the honey is collected as shown by Plate 5. As the intensity of the solar
radiation from the sun increases, the viscosity of the content of the honey
comb reduces, while both honey and wax trickle down into the plastic basin
beneath until a great proportion of the content of comb is completely drained
off by the heat. The substance collected is left untouched until the next day
after which the bee wax must have hardened over the surface of the solution,
thereafter scrapped – off. The clear honey is then collected separately in
another plastic container.
Unfortunately, solar
melting method of honey extraction has the following limitations:
·
Vasyl (2003) reported that exposure to
excessive heat of over 370C results in the lost of health values of
honey via reduced antibacterial strength and the destruction of important
enzymes (such as diastase and invertase) activities
·
Lost of the honey’s nutritional values
and quality as excessive heat also affects its appearance (darkens the natural
honey colour, taste and fragrance (Subramanian et al., 2007).
·
The honey is contaminated by dust and
dirts and easily absorbs moisture in the air thereby enhancing the rapid
fermentation of the product.
Plate 5: Solar melting
method of honey extraction
2.1.5 SIEVING METHOD:
This method of honey extraction is very similar, in terms of set up, to the
solar melting method. Unlike the solar melting method which makes use of woven
basket made of palm leaves, and solar radiation from the sun to facilitate the
ejection of honey from honey comb, the sieving method utilizes set of sieves of
wired-net configurations ranging from coarse particle sized to very fine
particles size openings. The sieves are arranged in a concentric form, the
finest mesh being on the outside and coarser on the inside. The entire process
is done in-door under room temperature (180 – 230c). Thus
after chopping the decapped honey comb into smaller pieces, they are poured
into the uppermost sieve with the biggest particle size configuration in the
set of sieves set – up, in vertically downward descending order; in terms of
particle size configurations. A plastic container is placed under the set of
about four sieves, as shown by Plate 6, to collect the pure honey which falls
solely by the force of gravity acting on the comb. This set – up is usually
left undisturbed for at least three days depending on the viscosity of the
product. This method of honey extraction poses less risk of contamination to
the product, unlike the solar melting method.
Plate 6: Sieving method of honey extraction
However, the sieving method of honey extraction has
its own limitations as follow.
·
It is time consuming
·
The sieve set up can accommodate only
small quantity of honey comb for extraction process at a given time
·
The honey can easily absorb moisture
from the air when left exposed for too long
2.2
QUALITY
AND QUALITY CONTROL OF HONEY
Quality
is defined as the degree of excellence which a material possesses (Guralink,
1975). Solabi (1985) in his own submission perceived quality as what is needed
to satisfy consumers expectations at all times. Subsequently, Sanni (1997) viewed
quality as the totality of features and characteristics of a product or
services that bears on its quality to satisfy stated or implied needs. Thus, according
to Oyinlola (2004), “Quality control” in food processing plants involves using
quality inputs; raw and packaging materials that satisfy product
specifications, standard manufacturing practices, proper laboratory analysis of
samples taken at critical control points, good storage and shipping schedules
for both the raw materials and the finished product.
The
quality control of honey therefore, is built on two main principles, the first
is to verify the (honey) genuineness, that is, to reveal possible frauds such
as artificial honey and adulteration; and secondly, to determine its quality
with respect to the need of the processor and the market (Krell, 1996).
Undoubtedly, most of the challenges encountered with regards to the quality
control of honey emanate from the harvesting and extraction processes adopted
be it traditional or modern for the product. Hence, as a panacea to the
possible risks to honey quality by the unwholesome practices of some
traditional method of honey extraction, as highlighted earlier on by Adjare
(1990) and Mutsaers (1991), the Devon Apicultural Research Group (DARG) based
in the United Kingdom, suggested that all honey producing nations adopt a
process of analyzing and dealing with possible hazard; called Hazard Analysis
Critical Control Points (HACCP).Having a HACCP plan is compulsory for
commercial honey producers in developed countries (DARG, 2012).
2.3
QUALITY
PARAMETERS OF HONEY
Over
the years, several researches have been conducted on the different parameters
that govern the quality of honey. Some of the most important of these quality
parameters are as follow:
2.3.1 MOISTURE CONTENT: As reported by Scott
(2012), honey has a low availability of water for bacteria to use, being about
84% fructose and glucose. The 15 – 21% of water by weight in honey strongly
interacts with the sugar molecules and thus, there is very little left
available for anything else.
Hence,
Krell (1996) stated that only osmophilic (sugar – tolerant) yeasts can grow in high
sugar concentration, with their rate of multiplication increased proportionally
with increasing moisture content (usually above 18% moisture in 100g of honey. Thus, while Lawal et al., (2009) reported a moisture content of 19.6% for honey samples
sourced from Yola, North-East – Nigeria, the amount of moisture of honey, as
reported by other authors include 17.6% (SueBee, 2011); 34.7% in Jalingo,
(Agbagwa, et al., 2011), and 21.0%
(NIS, 2003).
2.3.2 pH: Honey pH is another property that makes
the product such a potent anti-bacterial agent. According to Scott (2012),
honey generally has a pH value between 3.2 – 4.5, making it a very acidic
agent. Most bacteria, as further stated by Scott (2012) need a less acidic environment
to thrive and propagate. For example, E. coli, Salmonella and Streptococci; all
need a pH environment of between 4.0 – 4.5 to flourish. Thus, the pH of some
honey samples as reported by some authors include 5.6 in Yola, (Lawal et al., 2009), 3.10 in Jalingo, (Agbagwa
et al., 2011) and 3.42 – 6.10 (NIS,
2003).
2.3.3 Ash Content: Lawal et al., (2009) defined honey ash content as a measure of the
mineral elements in honey. It indicates how good or bad the physical properties
of honey are and it is also a good criterion for determining honey botanical origin.
Therefore, the ash content of some honey samples as reported by some authors
include 0.80% in Yola, (Lawal et al.,
2009), 0.953% in Jalingo, (Agbagwa et
al., 2011), 0.17% (SueBee, 2011) and 0.60% (NIS, 2003).
2.3.4 Hydroxymethyl Furfural (HMF)
Content: HMF content indicates honey freshness and overheating.
HMF is a by-product of fructose decay which is practically absent in fresh
honey, but it (HMF) increases upon storage, depending on the pH of honey, and
on either the extracting or storage temperature. Hence, the presence of HMF is
considered as the main indicator of honey deterioration (Krell, 1996). Thus, in
international trade, a maximum value of 40mg per kilogram (kg) has proven
satisfactory, while the codex proposal is a maximum of 60mg/kg (Bogdanov et al., 2001). Also, we have 0.38mg/100g
for Yola, (Lawal et al., 2009) and
40.0mg/kg as maximum value by NIS (2003).
2.3.5 Total Acidity:
Honey, according to (Wilkins and Lu, 1995), contains many kinds of acids, both
organic and amino. Organic acids comprise most of the acids in honey,
accounting for 0.17 – 1.17% of the mixture, and they include gluconic, formic,
citric and lactic acids among a few. Honey, within the standard approved range
for total acidity allows for an enhanced shelve stability of the product and
thus, prevent spoilage by micro organisms (Williams et al., 2009). Total acidity as reported by other authors include
1.90g/ml (Agbagwa et al., 2011),
40.0mg/kg (NIS, 2003) and 29.12meq/kg (SueBee, 2011), and 0.04% lactic acid in
Yola, (Lawal et al., 2009).
2.3.6 Sugar Content: Honey is a mixture of sugars and other
compounds. With respect to carbohydrates, honey is mainly fructose (about
38.5%) and glucose (about 31.0%), making it similar to the synthetically
produced inverted (table) sugar syrup, which is approximately 48% fructose, 47%
glucose, and 5% sucrose (National Honey Board, 2012). Simple sugar particularly
fructose are responsible for most of the
physical and nutritional characteristics of honey (Krell, 1996) while the
presence of sucrose which constitute
1.3% of the dry matter in honey, provides information on adulteration and the
botanical origin of honey. For other authors, Fructose content include 34%
(Bidemi, 1999), 60% (Agbagwa et al.,
2011), 36.35% in Jalingo, (Agbagwa, et
al., 2011) and 38.38% (SueBee, 2011) .For Sucrose content: 1.8% (Agbagwa,et al.,2011),1.31%(SueBee, 2011) and
maximum, 5.0% (NIS, 2003). For Glucose content: 39.18% in Jalingo (Agbagwa et al., 2011).
2.3.7 Microbiological Characteristics:
The chief sources of micro – organisms in honey are the nectar of the flowers
and the honey bee (Lawal et al.,
2009). The microbiological parameters of honey include:
2.3.7.1Total Aerobic Mesophilic Bacteria
Plate Count (TPC): There is a risk of introducing micro
organisms into wounds, especially botulism (digestive system infection in
children under one year of age), if honey is used as a dressing agent (Postmes et al., 1995). The risk can be avoided
by sterilization via “Gamma Irradiation”. An international medical device
ingredient microbiological requirement for manufacturing is a TPC of less than
500cfu/g (Activon, 2013). Other authors’ report on the TPC of some honey samples
include: 1 x 103cfu/g (NIS, 2003) and 1.3 x 101cfu/ml in
Yola (Lawal, et al., 2009).
2.3.7.2Mould/Yeast Counts: Yeasts
have been shown to come from the nectar and from the intestinal content of bees
(Frazier and Westhoff, 1994). Honey is often spoiled by some osmophyllic yeasts
and moulds which are always present in honey, but they are unable to grow in it
and to change its composition if the sugar concentration is about 83% or
higher. The mould and yeast count as reported by some authors include: 1 x 103
cfu/g (NIS, 2003), and 1.3 x 101cfu/ml in Yola, (Lawal et al., 2009).
2.3.7.3E. coli and Coliform Count: Possible
spore – forming bacteria contamination of honey by micro organisms (examples,
coliform bacteria and pathogenic bacteria such as staphylococcus, salmonella
and clostridium species) are indicative of poor sanitary quality of honey
collection, extraction and storage conditions. Thus, the coliform count in freshly processed
honey, as presented by authors, is expected to read nil cfu/g (Activon, 2013),
nil cfu/g in Yola, (Lawal et al.,
2009) and nil cfu/g (NIS, 2003).
2.4
QUALITY
STANDARDS AND REGULATIONS FOR HONEY
Quality standards and regulations for most
commercial food products, as reported by Oyinlola (2004) is described as the
total sum of activities, observations (physical and instrumental examinations)
and other measures employed to ensure that a uniform standard of excellence is
attained and maintained for all batches of the food products, manufactured at
all times. Thus, Oyinlola (2004) further stated that a key tool to assure
quality in any finished manufacture food such as honey is the “Product Standard
Document”.
Consequently in Nigeria, however, the quality standards
governing the regulation of honey production and marketing in the country as
specified by NIS 473: 2003 is presented in Table 1:
Table
1: Quality Requirements of Nigerian Honey
S/NO
|
CHARACTERISTICS
|
SPECIFICATION
|
1
|
Moisture
content (%) (max)
|
21.0
|
2
|
Ash
content (%) (max)
|
0.6
|
3
|
Specific
rotation (α)20 D
|
-20.4 to + 4.8
|
4
|
Total
acidity
|
40
milli-equivalent per 1000 grammes (max)
|
5
|
pH
|
3.42 – 6.10
|
6
|
Sucrose
content (%) (max)
|
5.0
|
7
|
Reducing
sugar calculated as invert sugar (%) (max)
|
0.5
|
8
|
Fructose/dextrose
ratio
|
106 – 119: 900
|
9
|
Water
insoluble content (pressed honey) (%) (max)
|
0.5
|
10
|
Water
insoluble content (unpressed honey) (%) (max)
|
0.1
|
11
|
Weight
per volume (g/litre)
|
1352 – 1500
|
12
|
Diastase
activity (diastase figure on gothe scale) (max)
|
8
|
13
|
Hydroxymethyl
furfural content (mg/kg) (max)
|
40.0
|
14
|
Fiehes
test (detection of technical sugar)
|
Negative
|
15
|
Proline
content (mg/kg) (min)
|
180.0
|
|
Microbiology
|
|
a
|
Total
aerobic mesophilic bacteria plate count (cfu/g) (max)
|
1.0 x 103
|
b
|
Mould/yeast
count (cfu/g) (max)
|
5.0 x 101
|
c
|
Coliform
count (cfu/g)
|
Nil
|
d
|
E.
coli count (cfu/g)
|
Nil
|
|
Metallic contaminants
|
|
|
Arsenic
(As) (mg/kg) (max)
|
1.0
|
|
Copper
(Cu) (mg/kg) (max)
|
2.0
|
|
Lead
(Pb) (mg/kg) (max)
|
0.5
|
Source: Standard Organization of Nigeria: Nigeria
Industrial Standard (Standard for Honey) (NIS 473: 2003). ICS 67.180.10.
CHAPTER
III
RESEARCH
PROCEDURE
3.1 DESCRIPTION OF LOCATION
Twelve
(12) different commercial honey samples extracted using five (5) different
traditional methods, were sourced from eight (8) selected honey bearing
communities within Kaduna State, North-Western Nigeria; namely Ankwa, Doka,
Giwa, Kafancha, Katari, Kukui, Mando and Sabon Gari communities. The selected
honey-bearing communities are situated in the following Local Government Areas
(L.G.As) of Kaduna State:
Ankwa,
Doka and Katari communities (Kachia L.G.A);
Kafancha community (Zango Kataf L.G.A); Kukui community (Kagarko L.G.A);
Giwa community (Giwa L.G.A); Mando community (Igabi L.G.A) and Sabon Gari community
(Sabon Gari L.G.A).
Thus,
the sources of honey samples according to their sample labels were: Ankwa (sample
label A2), Doka (sample labels D2 and E1), Kafancha (sample label E2), Katari
(sample labels D1,F1 and F2), Kukui (sample label B2), Mando (sample label C2)
and Sabon gari (sample labels A1 and C1), respectively.
3.2 HONEY
SAMPLING METHODS
Twelve
(12) different commercial honey samples labeled; A1,B1,C1,D1,E1,F1, A2,B2,C2,D2,E2
and F2, extracted from their respective honey combs using five different
traditional methods of extraction; were obtained with the aid of
questionnaires, in the following order:
(i)
Floating method: (sample labels E2 and
F2)
(ii)
Honey pressing Method: (sample labels
A1,B1 and D2)
(iii)
Hand-squeezing method: (sample label
F1).
(iv)
Solar melting (Heating) method: (sample
labels A2, B2, C1andD1).
(v)
Sieving method: (sample labels C2 and
E1).
Having collected all the twelve (12) honey samples
in neat, well sealed plastic containers, as shown by Plates 7, they were all
stored on a wooden shelve in a dark room, under an average room temperature of
23oC, before being transferred to the laboratory for scientific
analysis of the samples’ quality parameters – as had been established by
several authors in chapter II. Therefore, the different laboratory analytical
methods adopted in the determination of the various quality parameters for all
the twelve commercial honey samples collected were as shown in Table 2.
Table 2: Laboratory Analytical Methods for Honey Sample
Parameters
ANALYTICAL
METHOD
|
QUALITY
PARAMETER DETERMINED
|
i.
Refractometry
ii.
Furnacing
(Decomposition)
iii.
Glass electrode
iv.
Titration of acidity
(Lactone hydrolysis)
v.
Quantitative analysis
vi.
Mathematical
equivalence
vii.
Mathematical
difference
viii.
Microbiological
Analysis,
-
Total plate count (TPC)
-
Mould / yeast count
-
Coliform count
-
E. coli count
|
Moisture
content
Ash
content
pH
Total
titrable acidity (% Lactic acid)
Sugar
(% glucose, fructose and sucrose) content
Density
(weight per volume)
Water
Insoluble content
Total
aerobic mesophilic bacteria
Mould
/ Yeast
Coliform
E.
coli
|
Plate 7: Honey sample collected for the study
3.3 LABORATORY ANALYSIS OF SAMPLES
Most
of the laboratory analytical methods adopted for the determination of the
quality parameters of all the twelve (12) commercial honey samples collected
were according to the harmonized methods of the International Honey Commission,
IHC (2009).
3.3.1 Determination
Of Moisture Content: The moisture content of the samples were determined by
the use of an Analogue Hand-Refractometer as shown by Plates 8a, and 8b which
serves a dual purpose, for moisture content (Range 12.0-27.0%) and total sugar
(Soluble solid) content (Range 58.0-90.0%) determination, under a maximum
sample temperature of 200C. A broom stick-drop from one sample was
placed on the glass slide of the refractometer after which the moisture level
was viewed via a lens in the direction of the reflection of the sun light. A
focusing ring on the refractometer was then employed in obtaining a real and
clearer reading of the moisture content on the moisture scale. Thereafter, the
residue of the observed sample was cleaned-off the glass slide of the refractometer,
and the same procedure was repeated for each of the remaining samples.
Plate 8 (a) & (b): Analogue hand-refractometer
3.3.2 Determination
Of Ash Content: An electronic digital VITCO Muffle Furnace with model
number; TC344 (SELEC), as shown by Plate 9 was employed in the determination of
the ash content of the samples. 5g of each sample was weighed-out separately, to
the nearest 0.001g, into twelve quartz ash dishes (or crucibles) that had been
pre-heated to remove any residual moisture from
the dish at low heat rising to between
350-4000C ashing temperature. Thereafter, all the dishes were cooled
in a dessicator to room temperature, and weighed to 0.001g. Thus, following the
preliminary ashing, all the dishes were placed in the pre-heated furnace and
then heated for at least 1hr before being cooled in the dessicator and weighed
again. The ashing procedure continued until constant weights were reached for
all the samples. The ash content of each sample was then calculated using the
mathematical expression:
Ash content (%)=
Plate 9:Digital muffle furnace
3.3.3 Determination Of pH: The pH of the samples
were determined by the use of an electronic digital pH metre with model number;
ORION 310, and range of 0.00-14.00. Prior to the use of the PH device, it was
calibrated using three (3) different Buffer solutions: buffer 4 (for acidity),
buffer 7 (for neutrality), and buffer 9 (for alkalinity). Thereafter, 10ml of
each honey sample was measured out separately into twelve (12) beakers and were
each diluted with 20ml of distilled water. The dilution was to lower the
viscosity of the samples so as to enable the sensitive device inside the glass
electrode of the pH meter to easily read the pH level of each honey sample, as
shown by Plates 10a and 10b, respectively.
Plate 10 (a) & (b): Digital pH meter
3.3.4 Determination Of Total Titrable Acidity (% Lactic Acid): 25ml
of each honey sample was diluted with 25ml of distilled water, and each
solution was then titrated separately against 0.1N NaoH (0.1 Normality sodium
hydroxide solution) using 0.25ml phenolphthalein as an indicator as shown by
Plate 11. The relative amount of lactic acid was determined using the
mathematical formula:
Lactic acid (%)=
Plate 11: Determination of total titrable acidity
3.3.5 Determination
Of Sugar (% Glucose, Fructose And Sucrose) Contents: The
specific quantity of the various sugars (glucose, fructose and sucrose) present
in each honey sample was determined using the method stipulated by the
Association of Official Analytical Chemists (AOAC) in the year 2006. Having
determined the total sugar (soluble solids) contents of each sample using the
same refractometry method as highlighted in 3.3.1, the constant standard sugar
concentration of each sugar (glucose, fructose and sucrose) content for all the
honey samples was prepared by dissolving 10g of each industrially prepared fine
sugar particles, separately, in 100ml of distilled water in three separate
conical flasks. Thereafter, the specific quantity of each sugar content present
in each honey sample was calculated using the following mathematic expressions:
Glucose content in sample=
x Total sugar content in sample
Fructose content in sample =
x Total sugar content in sample
Sucrose content in sample =
x Total sugar content in sample
Therefore,
the Reducing sugar content of each honey sample was calculated using the mathematical
expression; Reducing sugar content (%)= (Glucose content + fructose content) in
sample
3.3.6 Determination Of Density (Weight Per Volume):
The density of the honey samples was determined using the mathematical
equivalent method. The weight of 120mL (0.12L) of each sample was equated to
the weight of 1L of the same samples. The equivalent weight (g) per volume (L),
that is density of each sample was determined with the aid of an OHAUS Brain
weigh electronic digital Balance with model number: B500 and range of
0.00-550.00g as shown by Plate 12. Subsequently, the density of each sample was
calculated using the format of the mathematical expression for sample A1:
Weight
of sample A1: (g) per 0.12L = 164.74g
0.12L
= 1372.83g
Therefore,
the density of sample A1 was 1372.83 (g/L).hence, the sample procedure was
repeated for each of the remaining samples.
Plate 12: Digital weighing balance
3.3.7 Determination Of Water Insoluble Content:
The water insoluble content of the samples was determined by finding the
mathematical difference between the values of the total solids and the soluble
solids (total sugar content) of each sample. The value of the soluble for each
sample was obtained using the same procedure of the refractometry method as
highlighted in 3.3.1; the focusing_ring on the refractometer was employed in
obtaining a real and clearer reading of the soluble solids on the soluble
solids scale. Thus the water insoluble content of each sample was obtained
using the mathematical expression:
Total solids (%) =100 – Moisture
content
Water insoluble content (%) =Total
solids – soluble solids
3.3.8 Determination Of Microbiological Characteristics:
The microbiological analysis on the honey samples were carried out to determine
the magnitude of the presence of four (4) different groups of micro organisms
namely; Total aerobic mesophilic bacteria, Mould / Yeast, Total coliform and E.
coli. The culture media, which were collected in separate conical flasks and
also used for the analysis, were:
-
Plate count Agar, PCA (10g in 444mL
distilled water)
-
Eosine methylene Blue Agar, EMB (8.89g
in 250mL distilled water)
-
MacConkey Agar, MA (10g in 200mL
distilled water)
-
Potato Dextrose Agar, PDA (9.81g in
250mL distilled water)
-
Ringer tablet (1 piece in 500mL
distilled water)
-
Tartaric acid (2g in 9mL ringer solution
+ 11mL distilled water + 10g per 444mL PCA solution).
The
procedures for the complete analysis were as follow:
3.3.8.1 All the culture media solutions and
other glass wares to be used for the analysis were sterilized at a temperature
of 1210C under a pressure of
about 0.105MPa for 15 minutes in an Autoclave [SURGIFRIEND pressure steam
sterilizer; Model number: SM 280E, Range: for temperature (36-1380C),
for pressure (0.01 – 0.25 Mpa)] as shown by Plate 13.
Plate 13: Pressure – steam sterilizer
3.3.8.2 Thereafter, a serial dilution in two
levels, 101 and 102, was carried out on all the honey
samples by pipetting 1mL of each sample into 9mL each of the sterilized ringer
solution in separate test tubes. The resulting solutions were thoroughly mixed
and labeled as first dilutions such as: A1101; A2101;
B1101; B2101; … F1101 and F2101.
3.3.8.3 Similarly, 1mL out of each first
dilution was pipetted into another 9mL each of sterilized ringer solution in
separate test tubes. The resulting solutions were thoroughly mixed and labeled
as second dilutions such as: A1102,A2102,B1102,B2102…,
F1102 and F2102.
3.3.8.4 Subsequently, 4mL was pitetted out
of each first dilution out of which, also, 1mL each was poured into another set
of four separate petric dishes labelled according to each honey sample such as:
A1101 (dishes PDA, PCA, MA, and EMB), A2101 (dishes PDA,
PCA, MA and EMB),…, F2101 (dishes PDA, PCA, MA and EMB).
3.3.8.5 Furthermore, 4mL was pipetted out of
each second dilution out of which, also, 1mL each was poured into another set
of four separate petric dishes labelled according to each honey sample such
as:A1102 (PDA, PCA, MA and EMB), A2102 (dishes PDA, PCA,
MA, and EMB),…, F2102 (dishes PDA, PCA, MA and EMB).
3.3.8.6 Thereafter, the volume of each of
the four culture media_PDA, PCA, MA and EMB_was divided by 24 samples after
which the resulting volume for each culture media was poured into its
designated petric dishes for the first and second dilutions.
3.3.8.7 Afterwards, all the petric dishes
containing the culture media were incubated appropriately as follow:
·
PCA: The dishes (plates) were incubated
at 370C for 24-48hr
·
MA and EMB: The plates were incubated at
350C for 24-48hr
·
PDA: The plates (dishes) were incubated
at 300C for 24hr for yeast isolates and 3-5 days for moulds.
Following the incubation period and
the colony-forming unit counting processes for selected organism-carrying
plates (dishes), the counted isolated organisms were identified using the
Gram’s Staining Techniques, as follow:
3.3.8.8 A smear was prepared from a 24hour
old culture of isolated organism, as shown by Plates 14a and 14b, for each culture sample plate, on a clean
slide and allowed to air dry, after which the back surface of the film was
passed gently through heat (naked flame) thrice.
Plate
14(a) & (b): Identification of test media
3.3.8.9 Thereafter the film was placed on a
staining rack and then flooded with crystal violet solution and was allowed to
act for 1 minute before it was later rinsed with water and allowed to air dry.
3.3.8.10Gram
iodine solution was then applied on the film and allowed to act for 1 minute
before being rinsed again with water and allowed to air dry. Acetone was then
applied on the film and allowed to act for 5 seconds before being rinsed
immediately with water and allowed to air-dry.
3.3.8.11Sarfranine
solution was applied on the film and allowed to act for 30 seconds before being
rinsed with water and allowed to air dry, after the back surface of the slide
had been blotted with blotting paper.
3.3.8.12Finally,
a drop of oil immersion was applied on the film and the film was observed with
the oil-immersion-objective (lens) of a microscope, thereby identifying the
isolated organisms on the film, as shown by Plates 15a and 15b, respectively.
Plate 15 (a) and (b): Identification
of isolated organisms after gramm’s
staining test using microscope
3.4 METHOD
OF DATA ANALYSIS
To
have a quick analysis of data and a better understanding of results, all data collected were analysed using statistical
tools namely; Percentages, and Analysis of Variance (ANOVA) for two-factor
experiment for testing the formulated hypotheses, the two factors being the
methods of extraction and the quality parameters of the honey samples under
study; as stipulated by Murray and Larry (2011).
3.4.1 HYPOTHESES TESTING:
(a)
Null Hypothesis (Ho):
Ho(1): There is no
significant difference among the different methods of extraction.
Ho(2): There is no
significant difference among means of the quality parameters.
(b) Alternative Hypothesis (Hi):
Hi(1): There is
significant difference among the different methods of extraction.
Hi(2): there is
significant difference among the means of the quality parameters.
3.4.2 LEVEL
OF SIGNIFICANCE (¥)
5% or 0.05 level of significance (¥
= 0.05) was used for the hypotheses testing under a F- distribution table (Ftab).
3.4.3 DECISION
RULE
Reject null hypothesis, H0 (1)
or H0(2) or both, if F-calculated value (Fcal) is
greater than the F-table value (Ftab). Thereby, accepting the alternative
hypothesis, Hi (1) or Hi(2) or both, as the case may be. Otherwise, do
not reject.
ANALYSIS OF VARIANCE (ANOVA) TABLE
The ANOVA table for two-factor
experiment, as stipulated by Murray and Larry (2011), was constructed in the
format of Table 11 below:
Table
11: ANOVA Table-Format For Two- Factor Experiment.
Variation
|
Degrees
of freedom
|
Mean
Square
|
F
|
Between rows (methods of extraction)
VR=
|
a-1
|
|
(a – 1) and
(a – 1) (b – 1) degrees of freedom
|
Between columns (quality parameters)
VC=
|
b-1
|
|
|
Residual or error
VE= V-VR-VC
|
(a-1) (b-1)
|
|
|
Total V= VR + VC+
VE
=
|
ab-1
|
|
Where:
a=
number of factors (or treatments) on row
b=
number of factors (or treatments) on column
J
= entries on row (or methods of extraction)
K=
entries on column (or quality parameters)
T=
total of all entries
Tj= total of entries in the jth row
T.k=
total of entries in the kth column
V=
total variation (or total sum of square)
VR=
variation between rows (or methods of extraction)
VC=variation
between columns (or quality parameters)
VE=
variation due to error (or residual)
X2=
square of entries
å=
summation of entries within a range
F=
F-distribution calculated value (or F cal)
CHAPTER
IV
RESULT
AND DISCUSSION
4.1 PRESENTATION OF RESULTS
Honey
samples extracted using Floating (labels E2 and F2), Honey Pressing (labels A1,
B1 and D2), Hand- Squeezing (labels F1), Solar Melting (labels A2, B2, C1 and
D1) and Sieving (labels C2 and E1) methods had percentage moisture content of
19.00, 20.40.17.40, 16.80, 19.00, 22.00, 17.50, 17.40, 17.70, 20.00,15.50, and
18.90, respectively (Table 3), while the total sugar content (soluble solids)
of the samples were 79.50, 78.00, 81.00 81.50, 79.70, 76.70, 80.80, 81.00,
80.80, 78.40, 83.00 and 79.80 (Table 3).
The
percentage total solids of the honey samples extracted using Floating, Honey
Pressing, Hand-squeezing solar melting and Sieving methods were 81.00, 79.60,
82.60, 83.20, 81.00, 78.00, 82.50, 82.60, 82.30, 80.00, 84.50, and 81.10(Table 4),
while the percentage water insoluble content of the samples were 1.60, 1.60,
1.60, 1.70, 1.30, 1.30, 1.70, 1.60, 1.50, 1.60, 1.50, and1.30 respectively
(Table 4).
The
percentage ash content of the honey samples extracted using Floating, Honey
Pressing, Hand- squeezing, Solar Melting and Sieving methods were 0.60, 0.70,
0.65,0.70, 0.80, 0.75, 0.50, 0.85, 0.60, 0.70, 0.75 and 0.75 (Table 5). The honey
sample also had pH values of 4.03, 3.94, 4.16, 4.09, 4.11, 3.86, 3.84, 3.77,
3.44, 4.01, 3.77 and 4.15, respectively
(Table 5). The total titrable acidity calculated as % lactic acid of the
honey samples showed that samples extracted using Floating, Honey Pressing,
Hand-Squeezing, Solar melting and Sieving methods had percentage lactic acid of
0.22, 0.20, 0.12, 0.14, 0.23, 0.32, 0.21, 0.23, 0.13, 0.14, 0.37 and 0.24
(Table 6), the density (grammes per liter) of the samples were1347.56, 1322.35,
1372.83, 1372.58, 1331.18, 1382.16, 1329.50, 1363.75, 1351.44, 1336.25, 1359.92
and 1341.85 respectively (Table 6). While the percentage sucrose content of the
honey samples extracted using Floating, Honey Pressing, Hand- Squeezing, Solar-melting
and sieving methods were 27.58, 27.06, 28.10, 28.27, 27.65, 26.61, 28.03,
28.10, 28.03, 27.20, 28.80 and 27.69 (Table 7); the percentage reducing sugar
content of samples were 51.92, 50.94, 52.90, 53.22, 53.04, 50.08, 52.76, 52.90,
52.76, 51.20, 54.20 and 52.12 respectively (Table 7).
The
microbiological analysis of the honey samples extracted using Floating, Honey
Pressing, Hand-Squeezing Solar- Melting and sieving methods revealed that E.
Coli counts were absent from all honey samples. Total aerobic mesophilic
bacterial plate count (TPC) of samples were 4.5x103, 7.8x103,
9.0x103, 9.8x102, 4.1x103, 5.1x103,
8.0x103, 3.1x102, 1.7x102, 9.8x103,
7.2x102 and 6.2x103 colony forming units per gramme (cfu/g)
(Table 8). The colony forming units per gramme of mould and yeast count of
honey samples were 1.5x103, 7.0x101, 4.0x101,
3.0x102, 3.0x102, 4.0x102, 6.0x101,
3.0x102, 6.0x101, 2.0x101, 1.2x102
and 3.0x102, respectively
(Table 9), while the colony forming units per gramme of coli form count of
honey samples were 3.5x102, 5.5x102, 6.0x102,
1.6x103, 1.5x102, 1.3 x122. 7.7x103,
4.7x102, 9.5x102, 7.2x102, 1.6x103,
and 6.0x102 respectively (Table 10).
4.2 STATISTICAL ANALYSIS
All
data collected were analysed using Percentages and Analysis of Variance (ANOVA)
for two- factor experiments, as
stipulated by Murray and Larry (2011), for testing the formulated hypotheses _ Null
hypotheses, Ho(1), and Ho(2),
and the Alternative hypotheses, Hi(1) and Hi(2)
_as was earlier stated under section 3.4.
4.2.1 TABLE OF DATA AND COMPUTATION OF RESULTS
The
percentage means of data of the two factors under study are shown in Table 12.
Table 12: The Mean Results of the
Methods of Extraction and The Quality Parameters of Honey Samples.
|
|||||||
Method of
Extraction
|
Ash content
|
Lactic acid
|
Moisture content
|
Water insoluble content
|
Sucrose content
|
Reducing sugar
|
Total
|
Floating
|
0.65
|
0.21
|
19.70
|
1.60
|
27.32
|
51.43
|
100.91
|
Honey Pressing
|
0.72
|
0.16
|
17.73
|
1.53
|
28.01
|
53.05
|
101.20
|
Hand Squeezing
|
0.75
|
0.32
|
22.00
|
1.30
|
26.61
|
50.08
|
101.06
|
Solar-Melting
|
0.66
|
0.18
|
18.15
|
1.60
|
27.84
|
52.41
|
100.84
|
Sieving
|
0.75
|
0.31
|
17.20
|
1.40
|
28.25
|
53.16
|
101.07
|
Total
|
3.53
|
1.18
|
94.78
|
7.43
|
138.03
|
260.13
|
505.08
|
From
Table 12 the following results can be computed:
a
=5
b
= 6
T
= 100.91+ 101.20 + 101.06 + 100.84 + 101.07 =505.08
VE = V – VR – VC
\
VE = 10674.39 – 1700.72 – 7458.50 = 1515.17
Having
computed the results, the ANOVA table is constructed according to the format
presented in Table 11 under section 3.4.4, as shown in Table 13 below.
Table
13. Analysis of Variance Table For Computed Results
Variation
|
Degrees
of freedom
|
Mean
square
|
F
|
Between rows (methods of extraction)
VR =
1700.72
|
4
|
S2R =425.18
|
S2R / S2E
=5.61
with 4 and 20 degrees of freedom
|
Between columns (quality parameters)
VC = 7458.50
|
5
|
|
S2R / S2E
19.69 with 5 and 20 degrees of freedom
|
Error or residual
VE =
1515.17
|
20
|
|
|
Total
V= 10674.39
|
29
|
|
In
order to obtain the table values of the F – distributions in table 13, the
following expressions were employed:
Table
value of F – distribution (F tab); from Table 14,
F
tab = F¥, V1,
V2
Where:
F
tab = table value of F- distribution
F
¥
=
level of significance for the F- distribution; where ¥
=
0.05
V1
=
degrees of freedom for treatment (or factors)
V2
=
degrees of freedom for error (or residual)
Therefore,
-
Between rows (methods of extraction).
F tab = F 0.05, 4,
20 =
2.87
-
Between columns (quality parameters);
Ftab = F 0.05, 5,
20 =
2.71
From the statistical analysis carried –out, the
results revealed that the values of F – distribution calculated (F cal)
for both factors (or treatments; methods of extraction and quality parameters)
are greater than their table values (F tab) obtained. Consequently,
these imply that significant difference exists among the methods of extraction
in the analysis of variance with respect to the means of the quality parameters
of honey samples which, likewise, did significantly differ.
Thus, the null hypotheses, Hi(1) and Hi(2)
are rejected while, the alternative
hypotheses, H10 and
H20 hold through. Hence, the traditional methods
of honey extraction have significant impact on the quality parameters of the
honey samples in this study.
4.3 DISCUSSION
Results of the moisture content of honey samples in
this study, obtained using different traditional methods of honey extraction
(Table 3), revealed that all the samples, except sample labelled F1 (Extracted
using hand – squeezing method), were within the acceptable range (15.00 –
21.00%) as stipulated by NIS (2003) and Scott (2012). Honey samples labelled B1
(extracted using honey – pressing method) had the lowest moisture content (15.50%),
while that of F1 (extracted using hand squeezing method) had the highest value (22.00%).
High level of moisture in honey samples is indicative of either adulteration,
mixing with water during extraction process or absorption of moisture during
open storage (Lawal, et al, 2009). According to Agbagwa, et al., 2011), low moisture content of honey, as recorded for most
samples in this study, forms the most important parameter of honey quality,
because it defects the product’s storage life, processing characteristics and
protects it from attack by micro-organisms. The water – insoluble content of
the honey samples, extracted using different traditional methods (Table 4),
were all outside of the acceptable range (0.1 – 0.5%) as required by NIS(2003).
The results revealed water- insoluble content with a range of between 1.30 and
1.70% for all the honey samples in this study. Bogdanov, et al. (2001) reported
that honey – wax is a major source of water – insoluble contamination and its
high presence in all the samples suggests poor filtration techniques of the
product by all the traditional methods of honey extraction in the area
investigated.
According to NIS (2003), the maximum content of 0.6%
is stipulated for honey ash level. This value is in contrast to the findings of
this study which showed that, other than honey samples labeled A2 (0.5%) and C1
(0.6%) (both extracted using solar – melting method) and E2 (0.6%) (extracted
using floating method,) all the honey samples extracted using different
traditional methods (Table 5), had an ash content range of between 0.65 and
0.85%; beyond the acceptable limit by NIS (2003). The ash content of honey
samples extracted using different traditional methods in Kaduna state indicate
fairly good physical property. The pH value, however, were also within the
acceptable range of between 3.42 and 6.10 (NIS, 2003) as revealed by Table 5.
The significance of pH at acidic range in foods can not be over – emphasized.
Lawal, et al. (2009) reported that such acidic range prevent the honey samples
from constant infection by various species of micro- organisms and thus, help
to ensure constant shelf – life for the honey samples. Thus, the acidic pH of
all honey samples extracted using different traditional methods in Kaduna
state, indicate they have good shelf – life.
Total titrable acidity, just like the pH at acidic
range, allows for an enhanced shelve stability of honey and, thus, prevents
spoilage by micro – organism (Williams, et
al., 2009). The total titrable acidity of honey samples in this study,
expressed in terms of percentage lactic acids (Table 6) was highest in sample
labelled C2 (0.37%) (extracted using sieving method) and least in sample labelled
A1 (0.12%) (extracted using honey – pressing method). However only four honey
samples were within the acidic range (0.04-0.19%), as reported by Lawal, et al., (2009). The implication of this
result is that, most of the honey samples extracted using different traditional
methods in Kaduna state are susceptible to attack by micro –
organisms and spoilage, despite having good pH level. Results of the density
(weight per volume) of honey samples in this study (Table 6), revealed half of
all the samples across all the different traditional methods of extraction were
below the acceptable range (1352 – 1500 g/L) as stipulated by NIS (2003). Low
density of honey samples suggests high amount of water – insoluble particles
(Bogdanov, et al., 2001); which
implies one out of every two honey samples extracted using any type of
traditional method in Kaduna state had been poorly filtered, or diluted with
other substances such as sugar-cane sugar or corn syrup to increase its
(honey’s) quantity for much profit during sales.
Determination of sugars in honey is a quality
criteria which is influenced by honey storage and heating; and thus, it is an indicator
of honey freshness, adulteration and overheating (Agbagwa, et al., 2011). The results obtained for glucose, fructose and
sucrose contents of honey samples in this study (Table 7) are in contrast to
the range required by NIS (2003) and international standards. According to the
proposal by the International Honey Commission (IHC), a minimum content of the
sum of glucose and fructose (apparent reducing sugars) is 60g/100g (or 60%) for
all blossom honeys, while sucrose has a maximum content of 5g/100g (or 5%),
(Bogdanov et al., 2001). Thus, the
non- conformity of the sugars in the
honey samples in this study with the stipulated standards suggests, that the
honey samples extracted using different traditional methods in Kaduna state have either been adulterated with sugar
– cane sugars or possibly overheated during extraction processes.
Micro – organisms in honey may influence the
stability of the product and its hygienic quality (Snowdon and Cliver, 1996).
Microbes of concern in post – harvest handling of honey, as further reported,
are those that are commonly found in the product (that is, yeasts and spore –
forming bacteria), those that indicate the sanitary or commercial quality of
honey (that is, Coliforms and yeasts), and those that are under certain
conditions could cause human illness. The microbiological analysis of the honey
samples in this study (Tables 8,9 and 10), therefore, revealed that non of the
samples is completely free of adulteration. This can be seen clearly in the
disparities between the results of enumeration of microbes in honey samples and
the permissible limit prescribed by NIS(2003). Despite the absence of E. coli
and yeast count in all the samples, only honey samples labelled B1 (extracted
using honey – pressing method), C1 and B2 ( both extracted using solar-melting method) and C2 (extracted using sieving
method) were below the NIS (2003) maximum Total Bacteria Plate count (TPC) of 1.0
X 103 cfu/g. There was an overwhelming amount of the bacteria;
Lactobacillus species, which was an indication of the high content of lactic
acid in most of the honey samples. Other than honey samples labeled A1
(extracted using honey pressing method), all of the samples exceeded the
NIS(2003) maximum mould count of 5.0 x101 cfu/g; recorded high
presence of the mould species. Most worrisome situation was in Total coliform
count (TCC) in which all the honey samples revealed presence of coliform
species; which is in sharp contrast to a complete absence, as stipulated by NIS
(2003). Thus, the poor Microbiological status of honey samples extracted using
different traditional methods in Kaduna state is a clear indication of poor
sanitary conditions and unhygienic quality of extraction processes.
Consequently, such honey samples when consumed consistently over time could
pose health risks; such as Botulism (digestive system disorder), and Honey intoxication
(symptoms include dizziness, weakness, excessive perspiration, nausea, and
vomiting), to humans (FDA, 2012 and The National Honey Board, 2012).
CHAPTER V
CONCLUSSION AND RECOMMENDATION
5.1 CONCLUSION
All the honey samples analyzed in this
study had good shelf life and fairly good physical properties. Despite having
these attributes, all of the honey samples contained high amount of
water-insoluble contaminants (mainly honey-wax), the samples had been
adulterated with other substances (possibly sugar-cane syrups), they had been
overheated and were highly susceptible to attack by micro-organisms and
spoilage. The presence of pathogenic organisms like the coliforms and
lactobacillus bacteria in the honey samples indicated the poor sanitary and
commercial qualities of the products. As such, these honey samples are not safe
enough for human consumption, neither as sugar substitute in confectioneries nor
as health enhancer in medicine. Therefore, the fact that the highest percentage
of honey samples extracted and marketed in different retail outlets in Kaduna
state are obtained using traditional methods of extraction, necessitates an
urgent need to monitor and assess the quality of any batch of the product
extracted, for the benefits of the health of the consuming public, and for the
good of the honey industry in Kaduna state.
5.2 RECOMMENDATION
In order to holistically address the
challenges posed by the traditional methods of honey extraction on the products
quality status in Kaduna state, the following suggestions are recommended for
prompt action by the authorities concerned;
5.2.1 All the commercial bee farmers and honey
producers in Kaduna state should be mobilized by the state’s ministry of
agriculture and water resources into forming a strong and formidable, Cooperative
Society for proper identification, representation and easy access for/to
cooperate supports.
5.2.2 More enlightenment and retraining on the
current trends in apiculture and honey production should be given to the local
commercial bee farmers and honey producers via their cooperative society by the
state’s rural agriculture extension agency, to ensure the production of safe,
wholesome and marketable honey.
5.2.3 Capital support, in form of grants or loans
at low interest rates and good enough repayment period should be given to the
local commercial bee farmers and honey producers, via their Cooperative
society, by the Nigerian Agriculture, Cooperative and Rural Development Bank (NACRDB) to
acquire honey friendly and compatible extraction equipment, and build standard
honey processing rooms or halls.
5.2.4 The Kaduna state government through a public
- private partnership should intervene in the establishment of honey monitoring
and quality assessment centers, alongside standard laboratories, in the major
honey bearing communities of the state to render services to the local
commercial bee farmers and honey producers at affordable cost.
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APPENDIX I
Table
3:
Total sugar (soluble solids) content and moisture content of honey samples
extracted using different traditional methods.
Sample
|
Method
of Extraction
|
Total
Sugar Content (%)
|
Moisture
Content (%)
|
A1
|
Honey
Pressing
|
81.00
|
17.40
|
B1
|
Honey
Pressing
|
81.50
|
16.80
|
C1
|
Solar
Melting
|
80.80
|
17.70
|
D1
|
Solar
Melting
|
78.40
|
20.00
|
E1
|
Sieving
|
79.80
|
18.90
|
F1
|
Hand-Squeezing
|
76.70
|
22.00
|
A2
|
Solar
Melting
|
80.80
|
17.50
|
B2
|
Solar
Melting
|
81.00
|
17.40
|
C2
|
Sieving
|
83.00
|
15.50
|
D2
|
Honey
Pressing
|
79.70
|
19.00
|
E2
|
Floating
|
79.50
|
19.00
|
F2
|
Floating
|
78.00
|
20.40
|
Table 4:
Total solids and water insoluble content of honey samples extracted using
different traditional methods.
Sample
|
Method
of Extraction
|
Total
Solids (%)
|
Water
Insoluble Content (%)
|
A1
|
Honey
Pressing
|
82.60
|
1.60
|
B1
|
Honey
Pressing
|
83.20
|
1.70
|
C1
|
Solar
Melting
|
82.30
|
1.50
|
D1
|
Solar
Melting
|
80.00
|
1.60
|
E1
|
Sieving
|
81.10
|
1.30
|
F1
|
Hand-Squeezing
|
78.00
|
1.30
|
A2
|
Solar
Melting
|
82.50
|
1.70
|
B2
|
Solar
Melting
|
82.60
|
1.60
|
C2
|
Sieving
|
84.50
|
1.50
|
D2
|
Honey
Pressing
|
81.00
|
1.30
|
E2
|
Floating
|
81.00
|
1.60
|
F2
|
Floating
|
79.60
|
1.60
|
APPENDIX
II
Table5:
Ash content and pH values of honey samples extracted using different
traditional methods.
Sample
|
Method
of Extraction
|
Ash
Content (%)
|
pH
values
|
A1
|
Honey
Pressing
|
0.65
|
4.16
|
B1
|
Honey
Pressing
|
0.70
|
4.09
|
C1
|
Solar
Melting
|
0.60
|
3.44
|
D1
|
Solar
Melting
|
0.70
|
4.01
|
E1
|
Sieving
|
0.75
|
4.15
|
F1
|
Hand-Squeezing
|
0.75
|
3.86
|
A2
|
Solar
Melting
|
0.50
|
3.84
|
B2
|
Solar
Melting
|
0.85
|
3.77
|
C2
|
Sieving
|
0.75
|
3.77
|
D2
|
Honey
Pressing
|
0.80
|
4.11
|
E2
|
Floating
|
0.60
|
4.03
|
F2
|
Floating
|
0.70
|
3.94
|
Table
5: Total
Titrable acidity (% Lactic Acid) and density (Weight per volume) of honey
samples extracted using different traditional methods.
Sample
|
Method
of Extraction
|
Total
titrable acidity (% Lactic Acid)
|
Density
(Weight per volume, g/L )
|
A1
|
Honey
Pressing
|
0.12
|
1372.83
|
B1
|
Honey
Pressing
|
0.14
|
1372.58
|
C1
|
Solar
Melting
|
0.13
|
1351.44
|
D1
|
Solar
Melting
|
0.14
|
1336.25
|
E1
|
Sieving
|
0.24
|
1341.85
|
F1
|
Hand-Squeezing
|
0.32
|
1382.16
|
A2
|
Solar
Melting
|
0.21
|
1329.50
|
B2
|
Solar
Melting
|
0.23
|
1363.75
|
C2
|
Sieving
|
0.37
|
1359.92
|
D2
|
Honey
Pressing
|
0.23
|
1331.18
|
E2
|
Floating
|
0.22
|
1347.56
|
F2
|
Floating
|
0.20
|
1322.35
|
APPENDIX III
Table 7:
Sugar (% Glucose, Fructose and Sucrose) contents and reducing sugar content of
honey samples extracted using different traditional methods.
Sample
Label
|
Method
of Extraction
|
Standard
Sugar Concentration in 100mL of Distilled Water
|
Sugar
Content in Sample
|
Reducing
sugar content (%)
|
||||
|
|
Glucose
(%)
|
Fructose
(%)
|
Sucrose
(%)
|
Glucose
(%)
|
Fructose
(%)
|
Sucrose
(%)
|
|
A1
|
Honey
Pressing
|
8.00
|
8.00
|
8.50
|
26.45
|
26.45
|
28.10
|
52.90
|
B1
|
Honey
Pressing
|
8.00
|
8.00
|
8.50
|
26.61
|
26.61
|
28.27
|
53.22
|
C1
|
Solar
Melting
|
8.00
|
8.00
|
8.50
|
26.38
|
26.38
|
28.03
|
52.76
|
D1
|
Solar
Melting
|
8.00
|
8.00
|
8.50
|
25.60
|
25.60
|
27.20
|
51.20
|
E1
|
Sieving
|
8.00
|
8.00
|
8.50
|
26.06
|
26.06
|
27.69
|
52.12
|
F1
|
Hand-Squeezing
|
8.00
|
8.00
|
8.50
|
25.04
|
25.04
|
26.61
|
50.08
|
A2
|
Solar
Melting
|
8.00
|
8.00
|
8.50
|
26.38
|
26.38
|
28.03
|
52.76
|
B2
|
Solar
Melting
|
8.00
|
8.00
|
8.50
|
26.45
|
26.45
|
28.10
|
52.90
|
C2
|
Sieving
|
8.00
|
8.00
|
8.50
|
27.10
|
27.10
|
28.80
|
54.20
|
D2
|
Honey
Pressing
|
8.00
|
8.00
|
8.50
|
26.02
|
26.02
|
27.65
|
53.04
|
E2
|
Floating
|
8.00
|
8.00
|
8.50
|
25.96
|
25.96
|
27.58
|
51.92
|
F2
|
Floating
|
8.00
|
8.00
|
8.50
|
25.47
|
25.47
|
27.06
|
50.94
|
APPENDIX
IV
Table
8:
Result of enumeration of Mesophilic Aerobic Bacteria Count (Total Plate Count,
TPC) of honey samples extracted using different methods
Sample
Label
|
Method
of extraction
|
Colonies
counted
|
Colony forming
unit per gramme (cfu/g)
|
Gram’s
Reaction
|
Organisms
isolated
|
||
A1
|
Honey
Pressing
|
90x102
|
9.0x103
|
Gram
positive short rods
|
Bacillus
species
|
||
B1
|
Honey
Pressing
|
98x101
|
9.8x102
|
Gram
positive rods in chain
|
Lactobacillus species
|
||
C1
|
Solar
Melting
|
17x101
|
1.7x102
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
D1
|
Solar
Melting
|
98x102
|
9.8x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
E1
|
Sieving
|
62x102
|
6.2x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
F1
|
Hand-Squeezing
|
51x102
|
5.1x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
A2
|
Solar
Melting
|
80x102
|
8.0x103
|
Gram
positive oval-shaped cells
|
Yeast
species
|
||
B2
|
Solar
Melting
|
31x101
|
3.1x102
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
C2
|
Sieving
|
72x101
|
7.2x102
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
D2
|
Honey
Pressing
|
41x102
|
4.1x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
E2
|
Floating
|
45x102
|
4.5x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
F2
|
Floating
|
78x102
|
7.8x103
|
Gram
positive rods in chain
|
Lactobacillus
species
|
||
APPENDIX
V
Table
9:
Result of enumeration of Total Coliform Count (TCC) of honey samples extracted
using different traditional methods
Sample
Label
|
Method
of extraction
|
Colonies
counted
|
Colony forming
unit per gramme (cfu/g)
|
Gram’s
Reaction
|
Organisms
isolated
|
||
A1
|
Honey
Pressing
|
60x101
|
6.0x102
|
Gram
negative rods
|
Coliform
species
|
||
B1
|
Honey
Pressing
|
160x101
|
1.6x103
|
Gram negative short rods
|
Coliform species
|
||
C1
|
Solar
Melting
|
95x101
|
9.5x102
|
Gram negative short rods
|
Coliform species
|
||
D1
|
Solar
Melting
|
72x101
|
7.2x102
|
Gram negative rods
|
Coliform species
|
||
E1
|
Sieving
|
60x101
|
6.0x102
|
Gram negative short rods
|
Coliform species
|
||
F1
|
Hand-Squeezing
|
13x101
|
1.3x102
|
Gram negative rods
|
Coliform species
|
||
A2
|
Solar
Melting
|
77x102
|
7.7x103
|
Gram negative rods
|
Coliform species
|
||
B2
|
Solar
Melting
|
47x101
|
4.7x102
|
Gram negative short rods
|
Coliform species
|
||
C2
|
Sieving
|
160x101
|
1.6x103
|
Gram negative rods
|
Coliform species
|
||
D2
|
Honey
Pressing
|
15x101
|
1.5x102
|
Gram negative short rods
|
Coliform species
|
||
E2
|
Floating
|
35x101
|
3.5x102
|
Gram negative rods
|
Coliform species
|
||
F2
|
Floating
|
55x101
|
5.5x102
|
Gram negative rods
|
Coliform species
|
||
APPENDIX
V
Table
10:
Result of enumeration of Mould and Yeast (mould and yeast count) of honey
samples extracted using different traditional methods.
Sample
Label
|
Method
of extraction
|
Colonies
counted
|
Colony forming
unit per gramme (cfu/g)
|
Culture
media characteristics
|
Organisms
isolated
|
A1
|
Honey
Pressing
|
4.0x101
|
4x101
|
Whitish
powdery colony
|
Mould
species
|
B1
|
Honey
Pressing
|
3.0x102
|
3x102
|
Whitish
–swampy –powdery colony
|
Mould
species
|
C1
|
Solar
Melting
|
6.0x101
|
6x101
|
Whitish
powdery colony
|
Mould species
|
D1
|
Solar
Melting
|
2.0x101
|
2x101
|
Whitish
powdery colony
|
Mould species
|
E1
|
Sieving
|
3.0x102
|
3x102
|
Whitish
powdery colony
|
Mould species
|
F1
|
Hand-Squeezing
|
4.0x102
|
4x102
|
Blackish
powdery colony
|
Mould species
|
A2
|
Solar
Melting
|
6.0x101
|
6x101
|
Whitish
powdery colony
|
Mould species
|
B2
|
Solar
Melting
|
3.0x102
|
3x102
|
Greenish
powdery colony
|
Mould species
|
C2
|
Sieving
|
1.2x102
|
12x101
|
Blackish
powdery colony
|
Mould species
|
D2
|
Honey
Pressing
|
3.0x102
|
3x102
|
Whitish
swampy colony
|
Mould species
|
E2
|
Floating
|
1.5x103
|
15x102
|
Blackish
and whitish –swampy – powdery colony
|
Mould species
|
F2
|
Floating
|
7.0x101
|
7x101
|
Blackish
and greenish powdery colony
|
Mould species
|
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