RESEARCH ARTICLE Open Access

A comparison of photographic, replication and
direct clinical examination methods for detecting
developmental defects of enamel
Ali Golkari1,2*, Aira Sabokseir2, Hamid-Reza Pakshir2,3, M Christopher Dean4, Aubrey Sheiham1 and Richard G Watt1

Abstract

Background: Different methods have been used for detecting developmental defects of enamel (DDE). This study
aimed to compare photographic and replication methods with the direct clinical examination method for
detecting DDE in children’s permanent incisors.

Methods: 110 8-10-year-old schoolchildren were randomly selected from an examined sample of 335 primary
Shiraz school children. Modified DDE index was used in all three methods. Direct examinations were conducted by
two calibrated examiners using flat oral mirrors and tongue blades. Photographs were taken using a digital SLR
camera (Nikon D-80), macro lens, macro flashes, and matt flash filters. Impressions were taken using additional-
curing silicon material and casts made in orthodontic stone. Impressions and models were both assessed using
dental loupes (magnification=x3.5). Each photograph/impression/cast was assessed by two calibrated examiners.
Reliability of methods was assessed using kappa agreement tests. Kappa agreement, McNemar’s and two-sample
proportion tests were used to compare results obtained by the photographic and replication methods with those
obtained by the direct examination method.

Results: Of the 110 invited children, 90 were photographed and 73 had impressions taken. The photographic
method had higher reliability levels than the other two methods, and compared to the direct clinical examination
detected significantly more subjects with DDE (P = 0.002), 3.1 times more DDE (P < 0.001) and 6.6 times more
hypoplastic DDE (P < 0.001). The number of subjects with hypoplastic DDE detected by the replication method
was not significantly higher than that detected by direct clinical examination (P = 0.166), but the replication
detected 2.3 times more hypoplastic DDE lesions than the direct examination (P < 0.001).

Conclusion: The photographic method was much more sensitive than direct clinical examination in detecting DDE
and was the best of the three methods for epidemiological studies. The replication method provided less
information about DDE compared to photography. Results of this study have implications for both epidemiological
and detailed clinical studies on DDE.

Background
Developmental defects of enamel (DDE) can be detected
and studied using microscopic and macroscopic meth-
ods. Macroscopic methods are especially important in
epidemiological studies. Direct clinical examination is
the most widely used method for detecting enamel
defects, while photographic and replication methods are
of special interest because of their suggested advantages

over direct clinical examination. None of these methods
are fully standardized as no single detailed method is
used by many researchers. The replication method used
by some dental anatomists, archaeologists and anthro-
pologists is not used by epidemiologists. The signifi-
cance of digital technologies, which have opened up
new horizons in almost all aspects of science, has been
relatively neglected in epidemiological studies of DDE.
Digital photography, which has been shown to have
high levels of success in caries detection [1], has only
been used in a few DDE studies.* Correspondence: aligolkari@yahoo.com1Dept. of Epidemiology and Public Health, University College London, UK

Full list of author information is available at the end of the article

Golkari et al. BMC Oral Health 2011, 11:16
http://www.biomedcentral.com/1472-6831/11/16

© 2011 Golkari et al; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons
Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in
any medium, provided the original work is properly cited.

mailto:aligolkari@yahoo.com
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Direct clinical examination is fast and cheap and all
surfaces of teeth can be examined. However, it has
many disadvantages such as observer bias and effects of
visual problems related to fatigue of the examiner.
Accuracy is highly dependent on cooperation of subjects
[2,3]. Direct examination was unreliable when multiple
indices were used or compared [4]. Direct visual exami-
nation of enamel can be done with or without tactile
examination of the enamel surface with a probe [5].
Examination may be conducted under natural light,
avoiding direct sunshine. When natural light is not
strong enough or when posterior teeth are being exam-
ined, a fibre optic light may be used [6]. Teeth may be
cleaned before the examination [7,8]. Polarizing filters
may be used to overcome the burn outs from strong
flashlight and to enhance the visual details of enamel
defects, especially when the extent of defects is more
important than their colour [9].
Photography has been used in some studies of tooth

and enamel defects [3,4,9-14]. Assessing photographs is
more objective than direct clinical examination. With
photography it is possible for all cases (even from differ-
ent geographic areas or examined at different times) to
be assessed under standard conditions by one person or
one group of examiners [11]. Photography facilitates ran-
domization and blinding, so observer bias can be avoided.
Photographs can be kept for future reassessment or
application of different approaches or indices [3,12]. On
the other hand, the disadvantages of photography are
cost, technical sensitivity and inability to use tactility.
Furthermore, with single photographs only labial surfaces
of incisors are recorded. Multiple views are needed to
view more teeth and/or more surfaces [3]. Some surfaces
or parts of a surface may be missed even in multiple
views. Some researchers have preferred to use conven-
tional photography with 35 mm film [3,4,13]. However,
digital photography provides better conditions to record
developmental defects of enamel. Digital photography is
cheaper and independent of developing negatives and
printing or projection. Most importantly, it gives the
photographer the opportunity to view each image imme-
diately and repeat it in case there is any problem with the
image, such as a burn-out caused by flash; or to take sev-
eral photos and choose the best one later [15].
Replicas of teeth may be used in both macroscopic

and microscopic studies of enamel defects. In this
method the whole cast is in one colour, so changes in
colour of enamel are not shown. But a replica of teeth
gives the observer better visibility to investigate hypopla-
sia, including small changes in the enamel surface [16].
This method also enables researchers to spend as much
time as needed and provides a dry specimen that can be
studied easily from different perspectives without worry-
ing about adjacent structures. Disadvantages of the

replication method are cost, time needed to make repli-
cas, and its sensitivity to technical methods. Even under
the best conditions some proximal surfaces may not be
well recorded. And, as stated above, it only displays
hypoplastic defects.
As the three methods differ in sensitivity in detecting

DDE, it is surprising that very few studies have com-
pared them [3,4,14]. No published epidemiological study
has compared the results of detecting DDE using the
replication method with the direct examination on a
population basis. Wong et al. (2005) used the Modified
DDE Index to compare the photographic and direct
examination methods and found kappa agreement
values from 0.79 to 0.85 between them for detecting
subjects with any DDE. They used one-view, three-view
and five-view photographic methods. The highest preva-
lence of subjects with DDE (36.6%) was, surprisingly,
obtained from their one-view method. It was close to
the prevalence obtained by the direct clinical method
(33.9%). The intra-examiner reliability of the photo-
graphic method (k = 0.81 to 0.88) was also close to the
direct examination method (k = 0.82) [3]. Ellwood et al.
(1996) used the TF (Thylstrup and Fejerskov) Index [16]
for their comparison and found a substantial agreement
between the two methods at subject level (k = 0.63). At
subject level, the prevalence obtained by photographic
method (44.9%) was close to that obtained by the direct
examination (41.4%) [14]. Sabieha and Rock (1998) used
both the Modified DDE Index and TF Index and
reported almost perfect agreement between the direct
examination and the photographic methods for both
indices (k = 0.91 and 0.83 respectively). They only
assessed maxillary central incisors [4].
Several clinical indices have been developed to cate-

gorize enamel defects based on their nature, appearance,
microscopic features or their cause. Some indices, such
as the TF Index [17], were introduced specifically for
fluorosis. Other indices are descriptive and include all
kinds of enamel defects including fluorosis. The Modi-
fied DDE Index [6] is a descriptive index derived from
the original Developmental Defects of Enamel Index
[18]. It covers all defects based on their macroscopic
appearance. However, the criteria for classification are
closely related with histo-pathological changes [19]. The
Modified DDE index was claimed to be a more practical
and comparable index in epidemiological studies. Its
extensive use and its high degree of validity and reliabil-
ity support that claim [6,20-22].
As there are few epidemiological studies comparing

the three methods of detecting DDE, the objective of
this study was to compare the ability of the digital
photographic and replication methods with the direct
clinical examination method to detect DDE in children’s
permanent incisors.

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Methods
The study was conducted on relatively newly erupted
permanent incisors in a sample of 8 to 10-year-old
school children of the city of Shiraz in the south of Iran.
Approval and ethical permission were obtained from
Iran’s National Ethical Committee in Medical Research
and the regional Educational Head Office. A representa-
tive sample of 335 primary schools children in grades 3
to 5 were first examined using the direct clinical exami-
nation method. Children were excluded from the study
if they were outside the age range, had one or more per-
manent incisors unerupted or partially erupted, or had a
fracture or restoration in their permanent incisors. Fifty
five children with DDE and another 55 children without
DDE were then randomly selected and invited to dental
clinics for further investigation using the photographic
and replication methods.
Upon arrival at the clinic the purpose and stages

involved in the study were explained in detail to the
parents. Parental consent was requested for taking
photographs and impressions. DDE of permanent inci-
sors were recorded based on the Modified DDE Index
[6] in all three methods. Results of assessing photo-
graphs and replicas were separately compared with the
results obtained from the direct examination.

Direct clinical examination method
Direct intra-oral clinical examinations were carried out
by 2 calibrated examiners in classrooms using natural
light, disposable mirrors and tongue blades. Teeth were
examined wet, but excess saliva and food debris was
removed with sterilized gauze when necessary. Each of
the two examiners checked the other examiner’s find-
ings on 1 in 10 random selected children to test the
inter-examiner reliability. Testing the intra-examiner
reliability was only possible if subjects were assessed
again under the same conditions in schools. Permission
for school re-visits was not granted.

The Photographic method
A Nikon D80 digital SLR (Single Lens Reflex) camera
with a 105 mm macro lens which provided a magnifica-
tion of 1:1 and a macro double flash was used. The
quality of photos was set on “JPEG FINE” and 5.2 mega
pixels. Speed and diaphragm were set on 60 and 32
based on the best results obtained from a pilot study of
13 children chosen from the same population.
Photographs were taken by two calibrated photogra-

phers with the child sitting on a dental chair and leaning
back to avoid movement during focusing and taking
photographs. Cheeks and lips were retracted so that all
12 anterior teeth and part of the upper and lower gums
were shown. An assistant helped with retraction of
cheeks in less-cooperative subjects. The child was asked

to close the incisors together edge to edge. This was
practiced a few times while holding a mirror in front of
their face before taking the photograph. Food debris and/
or excess saliva was removed with sterilized gauze when
necessary. A “one view” photograph was considered to be
acceptable as only incisors were assessed [3]. Photo-
graphs were taken by focusing on the centre of the 4 cen-
tral incisors. The camera was planed approximately 15
degrees above the perpendicular to the central incisors’
plane to minimize specula reflection and burn outs. Each
photograph was evaluated for acceptability and quality. If
not acceptable, the photograph was repeated.
Photographs were viewed randomly on a 17” flat free-

angle monitor with high resolution (1028 by 1024 pix-
els) using “Adobe Photoshop CS version 8.0” software.
Each photograph was assessed and scored independently
by two calibrated examiners. Each photograph was first
viewed as actual size based on the magnification ratio of
1:1 used when taking them. Then the examiner could
use the magnifier tool to enlarge the photo several
times. Some defects were clearer when using higher
magnifications but some others were better seen with
lower magnifications when the sharpness of components
was higher.
The examiners’ first records were used to assess inter-

examiner reliability. Disagreements between examiners
on coding a DDE were then solved by reassessment of
teeth by both examiners for the purpose of comparing
the photographic and direct examination methods. To
test the intra-examiner reliability in the photographic
method, each of the two examiners re-rated all photo-
graphs in a computer generated random order a year
after the original assessment.

The Replication method
Impressions were taken of the anterior teeth of children
using heavy body (putty) and then light body (liner) of
Affinis, an additional curing rubber base material made
by Coltène/Whaledent. The impressions were disin-
fected by soaking in sodium hypochlorite for five min-
utes and stored in individual bags away from heat,
direct sunshine and pressure. They were cast using hard
orthodontic stone. All casts were assessed for hypoplas-
tic defects by two calibrated examiners. All casts and
impressions were viewed using a pair of dental loupes
with a magnification of x3.5. Type of DDE detected in
replicas and impressions were also recorded using the
Modified DDE Index and its subcategories, as men-
tioned above. However, considering the fact that opaci-
ties were not detectable in this method, codes given to
detected DDE were limited to 7 (pits) and 8 (missing
enamel).
Similar to the photographic assessment, examiners’

first records were used to test the inter-examiner

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reliability in replication assessment and then disagree-
ments were resolved by discussion. However, in this
method impressions and casts were both reassessed and
compared. To test the intra-examiner reliability, casts
and impressions were reassessed by the two examiners a
year after the original scoring. Unlike the photographs,
avoiding bias by recognition of impressions and casts
was not possible. This occurred because replications
were not the same shape or colour and lacked a rando-
mised environment such as that done by computer in
the photographic reassessment. However, the time per-
iod between the first assessment and the reassessment
(one year) was long enough to assume it was not possi-
ble for examiners to remember their first scoring at the
time of the reassessment.

Comparison of methods
The number and percentage of children with DDE and
teeth with DDE detected by each method was calcu-
lated. The total number of DDE detected by each
method was also calculated as several defects may be
present on one tooth. Such calculations made it possible
to compare the results obtained by photographic and
replication methods with those of direct examination
method at individual, tooth, and lesion levels. All types
of DDE were included in comparison of direct examina-
tion and photographic methods. However, only hypo-
plastic defects were taken into account when comparing
the direct examination and replication methods as col-
our changes were not recorded in the replicas. Kappa
agreement was used to test reliability of methods and
the agreement between each of the two photographic
and replication methods and the direct examination
method. Two-sample proportion test was used to evalu-
ate if the prevalences obtained by the two methods were
significantly different. McNemar’s test was used to test
whether number of subjects or teeth with DDE detected
only by one method was significantly higher than the
other method. The data collection took place in Spring
2007. The reassessment of photographs and models was

done in Spring 2008. SPSS (Version 14) software was
used for analysis.

Results
The number of children examined at schools, invited to
clinics, had their photographs taken, and had impres-
sions taken of their teeth are shown in Table 1. Ninety
five of the invited 110 children attended the clinics.
However, some parents did not give consent for photo-
graphs or impressions to be taken. Photographs were
taken of 90 children (81.8% response rate). Therefore,
the direct examination and photographic methods were
compared based on these 90 children. Impressions were
taken of teeth of 73 children (66.4% response rate)
which were used for comparison of the replication and
direct examination methods.
Results of the inter-examiner and intra-examiner relia-

bility tests for each test are shown in Table 2. As
explained earlier, intra-examiner reliability was not
tested for the direct clinical method. The intra-examiner
reliability for photographic and replication methods are
the average of the two examiners. 14 disagreements
were found between the two examiners in assessing the
photographs. 10 of them (72%) occurred when one of
the examiners missed detecting or reporting a DDE on
a tooth with 2 or more defects. 2 disagreements (14%)
occurred when a diffuse opacity was coded as “lines” by
one examiner and as “patchy” by the other one. Two
other disagreements (14%) were based on colour of
demarcated opacities. Eight disagreements were found
in replication assessments, all being related to distin-
guishing a DDE from an artefact.

Table 1 Number of children in each part of study, by sex

Sex Were
examined
at schools

Were
invited
to clinics

Had
photographs

taken

Had
impressions

taken

Girls 177 56 48 42

Boys 158 54 42 31

Total 335 110 90 73

Table 2 Inter-examiner and average intra-examiner reliability levels of each method in detecting DDE

Type of DDE Method Sample
size

Inter-examiner reliability Intra-examiner reliability

Individual
level

Tooth
level

Lesion
level

Individual
level

Tooth
level

Lesion
level

All types
of DDE

Direct examination 38 0.90 0.84 0.81 - - -

Photographic 90 1.00 1.00 0.90 1.00 0.99 0.93

Replication - - - - - - -

Hypoplastic DDE Direct examination 38 1.00 0.91 0.91 - - -

Photographic 90 1.00 1.00 0.95 1.00 0.99 0.95

Replication 73 0.93 0.80 0.78 0.94 0.84 0.80

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The photographic method detected all cases with DDE
that were detected clinically, except one. Twenty cases
were only detected by the photographic method. The
photographic method detected 1.4 times more children
with DDE, 2.1 times more teeth with DDE, and 3.1 times
more DDE lesions than the direct examination method.
The photographic method also detected 4.5 times more
individuals with hypoplastic DDE, 5.9 times more teeth
with hypoplastic DDE, and 6.6 times more hypoplastic
lesions than the direct examination method (Table 3).
There was a moderate agreement (k = 0.48) between the
two methods in detecting cases with DDE at subject
level. The photographic method detected significantly
more DDE than the direct examination method for the
following: number of subjects with DDE (P = 0.002),
number of teeth with DDE (P < 0.001), number of sub-
jects with hypoplastic defects (P < 0.001), and number of
teeth with hypoplastic defects (P < 0.001). In addition to
detecting higher numbers than the direct examination,
the numbers detected only by the photographic method
were significantly higher than the numbers detected only
by the direct examination for all 4 tests (P < 0.001).
One hundred and one teeth (88% of those detected by

direct examination and 41% of those detected by photo-
graphic method) had DDE detected by both direct exami-
nation and photographic methods. Fifty four teeth (47%
of those detected by direct examination and 22% of those
detected by photography) were identically scored by both
methods. The number increased from 54 to 66 teeth
when similar subcategories, scores 1 and 2, 3 to 5, and 7
and 8, were combined. Scores 6 and 9 were not combined
with any other subcategory. At the lesion level, 56 DDE
lesions (46% of those detected by direct examination and
15% of those detected by photographic method) were
identically scored by both methods. The number
increased to 70 defects when similar subcategories were

combined. Diffuse opacities had the highest prevalence in
both methods.
In the 73 children who had impressions taken of their

teeth, the replication method detected 1.5 times more
children with hypoplastic DDE, 2.4 times more teeth
with hypoplastic DDE, and 2.3 times more hypoplastic
DDE lesions than the direct clinical examination method
(Table 4). 21 hypoplastic defects (87.5% of those
detected by direct clinical examination and 37.5% of
those detected by the replication method) were detected
by both methods. The prevalence of subjects with hypo-
plastic DDE was not significantly different between the
replication and the direct clinical examination methods
(P = 0.166). However, the proportion of teeth with
hypoplastic DDE detected by the replication method
was significantly higher than that obtained by direct
examination method (P < 0.001). On the other hand,
the number of affected subjects and teeth detected only
by the replication method were significantly higher than
those detected only by the direct clinical examination
method (P < 0.001).
The average time spent on direct clinical examination

of each child was about 3 minutes. Taking photographs
of each child, including the time spent for preparing the
child and repeating the photograph (if necessary) took
less than one minute. Taking impressions took 15 min-
utes on average. Examiners were told to spend as much
as time as they needed to assess the photographs and
replicas. Assessing a photograph took 6.5 minutes in
average. Assessing replicas took up to 20, and in aver-
age, 12 minutes.

Discussion
It was assumed that the photographic method would
detect more changes in colour and transparency of
enamel than the direct clinical examination method. But

Table 3 Comparison of direct examination and photographic methods in detecting all types of DDE and in detecting
hypoplastic DDE in permanent incisors of 90 children

Type of
DDE

Method Number and
percent of
subjects
with DDE

(%)

Number
and

percent of
teeth with

DDE
(% of all
examined
teeth)

Mean number of
teeth with DDE

per child in all 90
children

Mean number
of teeth with

DDE per
affected child

*Number
of DDE in
all 90

children

*Mean DDE
per child in

all 90
children

*Mean
DDE per
affected
child

*Mean
DDE per
affected
tooth

All types of
DDE

Direct
examination

50
(55.6)

115
(16.0)

1.3 2.3 121 1.3 2.4 1.1

Photographic
method

69
(76.7)

246
(34.2)

2.7 3.6 374 4.2 5.4 1.5

Hypoplastic
DDE

Direct
examination

11
(12.2)

20
(2.8)

0.2 1.8 24 0.3 2.2 1.2

Photographic
method

49
(54.4)

117
(16.3)

1.3 2.4 159 1.8 3.3 1.4

*Note: Some teeth had more than one DDE.

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the ability of the photographic method to detect hypo-
plastic defects, where defective enamel had the same
colour as its surroundings, was in doubt. The replication
method, on the other hand, although not showing
changes in colour, was assumed to better detect the
hypoplastic DDE than the other two methods as it was
the usual method used by dental anthropologists and
anatomists to find fine hypoplasias. Results of this study,
however, suggest that the photographic method was
good enough to detect both hypomineralized and hypo-
plastic enamel defects. The photographic method, whilst
not necessarily the most sensitive method, detected con-
siderably more DDE of all types, 3.1 times more DDE
lesions in total, than the direct examination method.
This study found only a moderate agreement (k = 0.48)

between the direct clinical examination and photographic
methods in detecting DDE at subject level. These find-
ings differ from other epidemiological studies comparing
the photographic and direct clinical examination meth-
ods. They reported kappa values of 0.63 [14] to 0.91 [4].
The low level of agreement found in this study was not
due to the inability of the photographic method to detect
DDE, but due to significantly more subjects with DDE
being detected by the photographic method than the
direct examination method (P = 0.002). Results of the
study by Ellwood et al. [14] also showed significant differ-
ences between the numbers of subjects with DDE
detected by the two methods, although they found a
much smaller difference. The other two studies men-
tioned above did not find such results [3,4]. Indeed they
reported very similar prevalence of cases with DDE
detected by the two methods. Wong et al. [3] reported
that 33.9% of their subjects had a DDE detected by the
direct examination with a very similar percentage of
34.6% to 36.6% detected by the photographic method.
The photographic method used in the present study was
able to detect most (98%) of the cases detected by the
direct examination method plus a significant number of
new cases. None of the three above-mentioned studies
reported a similar finding.

As with the comparisons at subject level, at the tooth
level the photographic method detected most of the
DDE detected by direct examination plus significantly
more other affected teeth. Comparing the results of the
present study with those of Sabieha and Rock [4] in
detecting a DDE in permanent upper central incisors,
both studies found that the photographic method
detected around 82% of those upper central incisors
detected by the direct examination (46 out of 56 in this
study, and 161 out of 194 in the study by Sabieha and
Rock). However, the percentage of affected upper cen-
tral incisors detected only by the photographic method
in the present study (27%) was three times greater than
the 9% reported by Sabieha and Rock [4] (P < 0.001).
These findings show that the photographic method

used in this study detected more DDE than both the
direct clinical examination method used in this study
and the photographic methods used in other studies at
both subject and tooth level. Unfortunately no previous
study compared the two methods at lesion level. The
main differences in the methods used in this study from
those used in the above-mentioned studies are that in
the present study a powerful digital camera with well
tested accessories and settings was used. That allowed
the photographer to zoom and focus to have the best
picture of the 8 incisors instead of using a fixed barrel
lens, and allowed the examiners to view the photographs
at different magnifications and angles, as they were able
to do during the direct clinical examination.
Both photographic and replication methods provided

permanent records of teeth, but the photographic
method also provided for easy random presentation of
subjects with less bias than in the other methods. The
photographic method was also faster than replicas, both
in time needed to be taken (1 versus 15 minutes) and in
time to be assessed (6.5 versus 12 minutes), with no
laboratory process and no concerns about cross infec-
tion. A clinical setting or presence of a dental clinician
was not necessary for taking photographs. Unlike the
photographic method, the replication method showed

Table 4 Comparison of direct examination and replication methods in detecting hypoplastic DDE in permanent
incisors of 73 children

Method Number and
percent of

subjects with
DDE
(%)

Number and
percent of
teeth with

DDE
(% of all
examined
teeth)

Mean number of
teeth with DDE per

child in all 73
children

Mean number of
teeth with DDE

per affected child

*Number of
DDE in all
73 children

*Mean DDE
per child in

all 73
children

*Mean
DDE per
affected
child

*Mean
DDE per
affected
tooth

Direct
examination

13
(17.8)

20
(3.4)

0.3 1.5 24 0.3 1.9 1.2

Replication
method

20
(27.4)

47
(8.1)

0.6 2.35 56 0.8 2.8 1.2

*Note: some teeth had more than one DDE in them.

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lower inter-examiner reliability levels than the direct
clinical examination method (Table 2).

Conclusion
The digital photographic method detected much more
DDE than the direct examination method and provided
much more information than the replication method.
Therefore, the digital photographic method, as used in
this study, was the best of three methods used for
detecting enamel defects of permanent incisors of chil-
dren. Results of this study have implications for both
epidemiological and detailed clinical studies on DDE.

Acknowledgements
The camera and its accessories were provided by the Borrow Foundation
(UK). Impression material was provided by the Coltène/Whaledent
(Switzerland). Authors would like to thank Drs Zahra Pakshir, Yasmin
Hadaegh and Hassan Abiri for their help in data collection.

Author details
1Dept. of Epidemiology and Public Health, University College London, UK.
2Dental School, Shiraz University of Medical Sciences, Iran. 3Orthodontic
Research Centre, Shiraz University of Medical Sciences, Iran. 4Dept. of Cell
and Developmental Biology, University College London, UK.

Authors’ contributions
This paper is based on a PhD thesis by AG done under the supervision of
RGW and ASh. ASa helped with data collection, processing and analysis. The
fieldwork was planned and supervised by HRP. MCD helped with the design
of the study and provided technical advice and support. AG wrote the
paper. All authors read and approved the final manuscript.

Competing interests
The authors declare that they have no competing interests.

Received: 2 September 2010 Accepted: 21 April 2011
Published: 21 April 2011

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Pre-publication history
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doi:10.1186/1472-6831-11-16
Cite this article as: Golkari et al.: A comparison of photographic,
replication and direct clinical examination methods for detecting
developmental defects of enamel. BMC Oral Health 2011 11:16.

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	Abstract
	Background
	Methods
	Results
	Conclusion

	Background
	Methods
	Direct clinical examination method
	The Photographic method
	The Replication method
	Comparison of methods

	Results
	Discussion
	Conclusion
	Acknowledgements
	Author details
	Authors' contributions
	Competing interests
	References
	Pre-publication history