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Addis Ababa University College of Health Sciences School of Allied Health Sciences Department of Medical Laboratory Sciences

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Addis Ababa University

College of Health Sciences


School of Allied Health Sciences
Department of Medical Laboratory Sciences

Prevalence of hepatitis B and C Viruses associated risk factors and knowledge,


attitude and practice among refugees at Pugnido-I camp in Gambela, Ethiopia.

BY: Abiyu Ayele (BSc)

Advisors:Kassu Desta (Associate professor, PhD fellow)

Melese Hailu (Msc,PhD fellow)

A research thesis submitted to the department of medical laboratory sciences, school


of allied health sciences, and college of health sciences, Addis Ababa University in
partial fulfillment of the requirements for the degree of Master of Science in clinical
laboratory science (diagnostic and public health microbiology).

June, 2018
Addis Ababa, Ethiopia

i
Addis Ababa University

School of Graduate Studies


This thesis prepared by Abiyu Ayele which is entitled Prevalence of Hepatitis B and C Viruses,
Associated Risk Factors and Knowledge, Attitude and Practice among refugees at pugnido-I
refugee camp in Gambela, Ethiopia. This is my original work and submitted for the partial
fulfillment of the requirements for the degree of Master of Sciences in Clinical Laboratory
Sciences (Diagnostic & Public Health Microbiology). It complies with the regulations of the
University and meets the accepted standards with respect to originality and quality. All sources of
material used for the thesis has been duly acknowledged.

Signed by the examining committee:

External Examiner:

Dr-Endale Hadgu (Assistant Professor PhD) Signature ___________Date _____________

Internal Examiner:

Dr-Aster Tsegaye (Associate professor, PhD) Signature ___________Date _______________

Advisors:

Mr-Kassu Desta (Associate professor,PhD fellow)Signature ____________Date_________

Mr- Melese Hailu (Msc,PhD fellow) Signature_____________ Date___________

_______________________________ Signature_____________ Date___________

Chairman of the department or Graduate program coordinator

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Acknowledgement

First of all I would like to thank the omnipresent and omnipotent God for giving permission to
perform day to day activities to do this project. Secondly, I would like to thank Addis Ababa
University College of health sciences school of allied health sciences department of medical
laboratory sciences for the opportunity to perform my thesis work. I would like to acknowledge
my advisors Mr-Kassu Desta and Mr-Melese Hailu for their guidance and valuable comments from
the point of topic selection to thus far and who made me stable and energize by giving first positive
response to writing the proposal and I would to acknowledge Mr-Muluken Birhanu for material
support.

I would like to thank my friend Mr-Dessie Abera for unlimited generate of an idea and technical
support during the projects, really thank you brother. I would also like to thank all instructors
participate in the lesson. Moreover, I would like to express my deepest gratitude to my wife
Mekdes Asrat for timeless support and encouragement to become this thesis fruitful. Last but not
least I would like to thank my study participants and office of administrative refugees and returnees
affaire (ARRA).

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Table of Contents
Acknowledgement ....................................................................................................................................... iii
List of Abbreviations ................................................................................................................................... vi
List of tables................................................................................................................................................ vii
Figure ......................................................................................................................................................... viii
Abstract ........................................................................................................................................................ ix
1. Introduction ............................................................................................................................................... 1
1.1. Background ........................................................................................................................................ 1
1.2 Statement of the problem .................................................................................................................... 3
1.3 Significance of the study ..................................................................................................................... 4
2. Literature review ....................................................................................................................................... 6
3. Objectives ............................................................................................................................................... 11
3.1. General Objective ............................................................................................................................ 11
3.2. Specific objective ............................................................................................................................. 11
4. Hypothesis............................................................................................................................................... 12
5. Materials and Methods ............................................................................................................................ 13
5.1. Study design and period ................................................................................................................... 13
5.2. Study area......................................................................................................................................... 13
5.3. Population ........................................................................................................................................ 13
5.3.1. Source of population ................................................................................................................. 13
5.3.2. Study population ....................................................................................................................... 13
5.4. Inclusion and exclusion criteria ....................................................................................................... 13
5.4.1. Inclusion criteria ....................................................................................................................... 13
5.4.2. Exclusion criteria ...................................................................................................................... 13
5.5. Study variables ................................................................................................................................. 14
5.5.1 Dependent variables ................................................................................................................... 14
5.5.2. Independent variables ............................................................................................................... 14
5.6. Sample size and sampling procedure ............................................................................................... 15
5.6.1 Sample size determination ......................................................................................................... 15
5.6.2. Sampling Technique ................................................................................................................. 15
5.7. Data collection and laboratory Analysis .......................................................................................... 15
5.7.1. Data collection .......................................................................................................................... 15
5.7.2. Laboratory analysis ................................................................................................................... 16

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5.8. Data entry and analysis .................................................................................................................... 18
5.8.1. Quality assurance and quality control ....................................................................................... 18
5.9. Ethical considerations ...................................................................................................................... 18
5.10. The overall work flow diagram ...................................................................................................... 19
5.11. Operational definitions................................................................................................................... 21
6. Results ..................................................................................................................................................... 22
6.1: Socio-Demographic Characteristics................................................................................................. 22
6.2. Prevalence of HBV and HCV .......................................................................................................... 23
6.3: Risk factors associated with prevalence of HBV ............................................................................. 24
6.4. Risk Factors associated with HCV prevalence ................................................................................ 26
6.5. Adjusted Odds Ratio of sex and age with prevalence of HCV ........................................................ 28
6.6. Knowledge, Attitude and Practices (KAP) assessment on HBV and HCV ..................................... 29
7. Discussions ............................................................................................................................................. 31
8. Strength and Limitation of the study...................................................................................................... 34
8.1. Strength of the study ........................................................................................................................ 34
8.2 Limitation of the Study ..................................................................................................................... 34
9. Conclusion and Recommendation .......................................................................................................... 35
9.1. Conclusion ....................................................................................................................................... 35
9.2. Recommendations ............................................................................................................................ 35
10. References ............................................................................................................................................. 36
Annexes ...................................................................................................................................................... 40
Annex-I. Information sheet ..................................................................................................................... 40
Annex - II. Consent Form ....................................................................................................................... 41
Annex - III. Questionnaire ...................................................................................................................... 42
Annex - IV. Laboratory Results format: ................................................................................................. 43
Annex - V. principle and procedure of tests ........................................................................................... 44
Annex .VI. Thesis declaration ................................................................................................................ 48

v
List of Abbreviations

CDC Centers for Disease Control and Prevention

CHB Chronic Hepatitis B

DNA Deoxyribose Nucleic Acid

ELISA Enzyme Linked Immunosorbent Assay

HAV Hepatitis A Virus

HBcAg Hepatitis B core Antigen

HBsAg Hepatitis B surface Antigen

HBV Hepatitis B Virus

HCC Hepatocellular Carcinoma

HCV Hepatitis C Virus

HDV Hepatitis D Virus

HEV Hepatitis E Virus

HIV Human Immunodeficiency Virus

KAP Knowledge, attitude and practice

MTCT Mother to Child Transmission

RNA Ribose Nucleic Acid

SNNPRs Southern Nations Nationalities and Peoples’ Regional States

SOPs Standard Operating Procedures

UNHCR United Nations High Commissioner of Refugees

WHO World Health Organization

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List of tables

Table 6.1.Socio-Demographic Characteristics among refugees…………………………………22


Table 6.2.Prevalence of HBV and HCV among refugees……………………………….............23
Table 6.3.RiskFactors associated with HBV infection …….…………………………...............25
Table 6.4.Risk Factors associated with HCV infection……………………………….................27
Table 6.5.Adjusted odds ratio for sex and age with HCV………………………………………28
Table 6.6.KAP assessment on HBV and HCV infection …………………………….................30

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Figure
Figure1.Work flow diagram of the study……………………………………………………...20

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Abstract
Background: In the last two decades Ethiopia has witnessed increasing immigration flows from
South Sudan, Somalia and Eritrea. However, these immigrants are not screened for hepatitis B and
C which could be additional burden for the local population.
Objective: To determine Prevalence of hepatitis B and C viruses, associated risk factors and
knowledge, attitude and practice (KAP) among refugees at Pugnido-I refugee camp in Gambela,
Ethiopia.
Methods: Cross-sectional study was conducted on 453 refugees at Pugnido-I refugee camp in
Gambella region from January to May 2018.Socio-demographic, risk factors and KAP was
assessed by using structured questionnaires. Five ml blood sample was collected with serum
separator tube. HBsAg and anti-HCV rapid screening tests were performed and those positive
samples were confirmed using ELISA method. Data was entered and analyzed using SPSS
statistical software version 20. The odds ratio and 95% confidence interval was calculated to assess
the strength of the association. P-value less than 0.05 were considered as statistically significant.
Results: The overall prevalence of HBV and HCV among refugees was 7.3 %( n=33/453) and 2.0
%( n=9/453) respectively. Of those 6.8% (n=25/370) and 1.4% (n=5/370) of females were positive
for HBV and HCV respectively. And 9.6 % (n=8/83) and 4.8 % (n=4/83) of males were positive
for HBV and HCV respectively There was no significant association between HBV and proposed
risk factors (p>0.05), however, statistical significant association was observed between HCV and
age group of 18-25years (AOR=0.045, CI 95%=0.005-0.378, P=0.004) and 26-35years
(AOR=0.035, CI 95%0.004-0.301, P=0.002). From the total participants, 86.5%(n= 392/453) did
not know how the disease is transmitted, 8.2%(n= 37/453) believed that hepatitis can be
transmitted through food, 86.8%(n= 393/453) had no information about the availability of HBV
vaccine and 98.5%(n=446/453) were not vaccinated.
Conclusion: The prevalence of hepatitis B and hepatitis C among refugees was intermediate which
might be due to low knowledge and attitude towards the transmission and prevention of the disease.
Therefore this indicates the need for creating awareness for refugees about the transmission and
prevention mechanisms of hepatitis B and hepatitis C infection. Large scale study is recommended
at national level.
Key Words: Hepatitis B virus, Hepatitis C virus, Pugnido Refugee camp, Gambella, Ethiopia.

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1. Introduction

1.1. Background
Hepatitis B, C and other viruses can cause hepatitis. It is clinically silent infections for decades
until developing cirrhosis, end-stage liver disease and hepato-cellular carcinoma. Hepatitis B and
C viruses can cause both acute and chronic infection [1]. Infection with hepatitis B and C virus
affects the liver and results in a broad spectrum of disease out come. An infection with HBV can
spontaneously resolve and lead to protective immunity, result in a chronic infection and, in rare
cases, cause acute liver failure with a high risk of dying [2].

HBV and HCV are transmitted by percutaneous or mucosal exposure to the blood or body fluids
of an infected person, from an infected mother to her newborn during childbirth, through close
contact within households, through exposures to unscreened blood transfusion or unsafe injections
in health care settings, through injection-drug use, and from sexual contact with an infected person
[1].

Refugee populations are more at risk of having sexually transmitted infections (STI), like HBV
and HCV. The contributing factors include: origin from countries that are highly endemic for these
infections, lack of information on hepatitis prevention directed to the migrant communities in the
host country. No screening takes place for infectious diseases of sexual transmission, though this
is recommended in the protocols of the Centers for Disease Control and Prevention [3]. Associated
risk factors of hepatitis B and C viruses; Occupational exposure to blood and body fluids, history
of sharp injury, blood donation family history of liver disease, tooth extraction, tattoo [4].

Diagnosis is based on clinical information and laboratory screening. HBV and HCV infection
cannot be differentiated on the basis of clinical symptoms alone, and definitive diagnosis depends
on the results of serologic testing such as rapid screening and ELISA [1].

About 350 to 400 million people infected with HBV due to this 1 million people deaths per year
and also 130 to 170 million people are infected with HCV that cause of about 350,000 deaths per

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year [5].The World Health Organization classifies countries according to the hepatitis B surface
antigen (HBsAg) into low (<2%), intermediate (2–8%), and high (>8%) prevalence [6].

Today, many people are obligated to leave their country and seek asylum in foreign countries due
to war and poverty, as well as to political, economic and social reasons in the last two decades
Ethiopia has witnessed increasing immigration flows from the different neighbor countries like
South Sudan, Somalia and Eritrea and others. Our public health policies are not focused on
screening immigrants for an infectious disease and no systematic actions against blood borne
diseases like hepatitis B and C are implemented [7].

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1.2 Statement of the problem

Viral hepatitis is the tenth leading cause of death and the leading cause of liver cancer worldwide
[6].About 85% of the world’s population live in areas of endemic of HBV such as intermediate
(2–7.9%) or high (> 8%).Some studies in specific populations indicated that prevalence of
infection ranging from 0.1% to 8%.Most individuals with chronic hepatitis B or C are unaware of
their infection status, because they can remain asymptomatic for year[8].About 350 and 80 million
people are estimated to have been chronically infected by HBV and HCV respectively and three-
to-four million new cases are detected each year [7].

About 3-4 million newly infected cases each year of HCV and a mean global sero-prevalence of
2.2-3.0%. Approximately 70% of those with acute infection develop chronic HCV infection and
20% of these individuals develop cirrhosis and 1-5% develops hepato-cellular carcinoma (HCC)
during the two decades following initial infection. There is no effective vaccination to prevent
against transmission of HCV. Chronic hepatitis C infection however, can easily detected through
widely available screening blood tests and standard treatment regimens are moderately
successfully (50% overall) in achieving sustained viral response (SVR) which in those with
cirrhosis decreases disease progression to liver failure and HCC [9].

Studies from the Horn of Africa, particularly Ethiopia, report a HBsAg carriage rate between 5.4
and 15% and anti-hepatitis C virus positivity between 0.8 and 5.1% in the different groups
Considered. Therefore, the arrival refugees may influence the prevalence of HBV and HCV among
the Ethiopian population, especially if no appropriate preventive programmed are planned [10].

During the last two decades, refugees from countries with an increased prevalence of infectious
diseases, such as viral hepatitis. The crowded living conditions and the avoidance of well-
organized places of sheltering, due to the fear of repatriation or expulsion, characterize immigrant
populations and facilitate the spread of these diseases [11]. In addition the increasing numbers of
immigrants from high to intermediate or low endemic regions forms a new dynamic epidemiology
of hepatitis transmission [12].

Increased migration volume and different hepatitis prevalence between immigration and
emigration countries have changed the Hepatitis viruses epidemiology considerably[13].As we

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know there are too many immigrants settled in Ethiopia from different neighbor countries mainly
originated from Somali, Eritrea, South Sudan and other countries. These immigrants cross the
border of the country without any health screening criteria and live at different refugee camps with
cohesion of the local people. Therefore, different disease can be transmitted from refugees to local
population unless extended health education and preventive mechanism planned in the country.
Moreover, these immigrants living system is not limited to in the camp rather highly
communicated to the local population no rule and regulation that restrict the movement of the
refugees through the local society. There are insufficient information about the prevalence of
hepatitis B and hepatitis C among refuges in Ethiopia. Therefore, this study was aimed to
determine the prevalence of hepatitis B and C virus among South Sudan refugees at pugnido-I
refugee camp Gambela, Ethiopia.

1.3 Significance of the study

This study provides the following information to the responsible bodies:

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 The study generates information on the prevalence of hepatitis B virus and hepatitis C virus
among refugees that helps health policy makers for designing appropriate intervention
strategies.
 This study gives information to the local responsible bodies to be aware about the disease
status among refugees to pay attention about the prevention of healthy population and
treatment the exposed individuals.
 Moreover, the finding of the study uses to formulate preventive mechanisms to halt the
spread of the disease to the local society as well as countrywide.
 Finally, the information obtained from knowledge, attitude and practice of participants
about the disease can give clue to the responsible bodies for planning health education
program based on the level of understanding of targeted group.

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2. Literature review

A cross-sectional survey conducted by Quddus A.et al, in Pakistan to estimate Prevalence of


hepatitis B among Afghan refugees living in Baluchistan. From a total of 903 Afghan refugees the
investigators found that 75 study subjects were positive for HBsAg. From which, 37 husbands, 21
wives and 17 children has been positive result for HBsAg. The prevalence of HBsAg among
Afghan refugees in Baluchistans Province was 8.3%, while the prevalence among husband, wife
and children were 12.3%, 7.0% and 5.6%, respectively. From their result they concluded that
vaccination is necessary for Afghanistan refugees [14].
Stevens K, et al conducted a cross-sectional study in India, to investigate hepatitis B prevalence
and treatment needs among Tibetan refugees residing; The investigators selected 2,769
participants, 945 (34.1%) were from households , 1,153 (41.3%) were from the boarding school,
and 671 (24.6%) were from the monastery. The assessment showed that from a total of
247 participants 8.9% were positive for HBsAg. Focusing just on the house hold sampling, 11.9%
were positive for HBsAg. And they generalized that vaccination of HBV is important to stop the
spread of infection [15].
Another study conducted by Hussein N R,et al, in Iraq to investigate Prevalence of HBV, HCV
and HIV Infections Among Syrian Refugees in Kurdistan Region. From a total of 880 refugees,
34 cases (3.86%) were positive for HBsAg. All samples showed HCV negative. From the local
people, 2,975 were volunteer to participate in the study of which, 30 (1.09%) were positive for
HBsAg and only one was positive for HCV.The investigators conclude that the prevalence of HBV
in Syrian refugees was nearly fourfold higher than that of indigenous people of Iraq[16].
The study conducted by Chironna M.et al in Kosovar 2001; Prevalence of Hepatitis Virus
Infections in Kosovar Refugees;The investigator Among the 526 Kosovar refugees, Among the
526 refugees, the prevalence of total anti-HAV antibodies was 81%. The prevalence of anti-HEV
antibodies was 25%. Fifteen subjects (2.9%) were positive for hepatitis B surface antigen
(HBsAg), whereas 17.5% tested positive for anti-hepatitis B core antigen (anti-HBc).Whereas
25.9% were found to be positive for anti-HBc. None of the refugees tested positive for anti-
HDV.The study group concludes that,an immunization policy against HBV infection, through
vaccination of all newborns and children before adolescence, may be advisable [17].

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A narrative systematic review conducted by Owiti J A, et al, in UK to assess Illness perceptions
and explanatory models of viral hepatitis B & C among immigrants and refugees. By using `51
publications.The studies focused on hepatitis B and ethnic groups of South East Asian immigrants
in USA, Canada, and Australia. Most immigrants lack of adequate knowledge of etiology,
symptoms, transmission risk factors, prevention strategies, and treatment, of hepatitis HBV and
HCV. The variation of knowledge becomes from Ethnicity, gender, better education, higher
income, and English proficiency. Immigrants are high risk to HBV and HCV, because of lack of
knowledge. The investigators conclude that, immigrants are vulnerable to HBV and HCV, because
of poor knowledge [18].
A cross-sectional study in UK by Evlampidou I,et al in titled by Low hepatitis B testing among
migrants. A total of 82 561 migrants who had informed to test HBV testing, 9627 (12%) were
‘HBV tested. The test coverage indicate that Eastern Africa 20%,Western Africa 15%, South
Eastern Asia 9%, Eastern Asia 5%.Of which born in UK 82 561 (17%)were identified with ≥2%
HBV prevalence. The investigators concludes that, much greater support for primary care and
awareness of national guidance are required[6].
The study conducted by Padovese V.et al in Malta with title of Prevalence of latent tuberculosis,
syphilis, hepatitis B and C among asylum seekers in Malta. The investigator selected 500 migrants
and screened for latent TB, hepatitis B, C and syphilis. Among them, 83.2% (n ¼ 416) were from
Somalia, 8.2%, from Eritrea, 2.4%, from Ethiopia and 5.6%, from West African countries. 81.2%,
were males and the mean age was 26.5 years. The study group suggests that, systematic screening
for asymptomatic migrants recommended for HBV but not HCV [10].
In Italy the study conducted by Coppola N, et al, to estimate Hepatitis B virus infections in
immigrant populations from different geographical regions such as South East Asia (0%-27.3%).
The HBsAg Seroprevalence in sub-Saharan immigrants ranged from 7.4% to 13.9%.High
prevalence were also observed in Albanian refugees two Greek studies, 11.7% and 15.3%,
respectively. The investigators concluded that the immigrant’s prevalence rose due to lack of
health care management, funds and follow up. The investigators conclude that, HBV vaccination,
good quality medical care and improved quality of life are the first steps [19].
Another study performed by Coppola N, et al, in 2017,to estimate Hepatitis B virus infection in
undocumented immigrants and refugees in Southern Italy, show that of the 1,212 immigrants
screened, 116 (9.6%) were HBsAg positive,490 were HBsAg negative/anti-HBc positive, and 606

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were seronegative for both. The investigators suggests that, provide screening, HBV vaccination,
treatment and education to immigrants [20].
The study conducted by Palumbo E, et al, in Italy, to determine prevalence of HBV-genotypes in
immigrants affected by HBV-related chronic active hepatitis. From a total 556 men participants
tested, 60 (10.7%) resulted HBsAg positive. From these 42 (70%) African 10 (16.6%) Asian and
9 (14.4%).In real-time PCR, Genotype distribution was as follow: genotype E, 16 (50%), genotype
D, 9 (28.1%), genotype A, 7 (21.9%).The study group concludes that, prevalence of HBV-
infection in immigrants, characterized by a different natural history and, a different response to
antiviral treatment[21].
The systematic review and meta-analysis by Greenaway C.et al, 2015 in Germany, a total of 973
titles and abstracts were screened, 173 full text articles were reviewed, and 50 were included in
this study. Immigrants account that 38635 which are around the world regions who arrived in
Australia, Canada, Europe, Israel and the United States. The study resulted in anti-HCV prevalence
of 1.9%.The investigators concluded, that adult migrants originating from Asia, Sub-Saharan
Africa and Eastern Europe are at high risk for HCV and may benefit from targeted HCV screening.
The investigators conclude that, migrants at increased risk for HCV have being benefit from
targeted HCV screening [22].
The study conducted by Roussos A.et al, in Athens 2003;Prevalence of hepatitis B and C markers
among refugees in Athens; The study group Twenty individuals (15.4 %) were HBsAg positive
and 69 (53.1 %) were anti-HBc positive. The prevalence of HBsAg and anti-HBc was higher
among refugees from Albania and Asia. The prevalence of these markers was found irrelevant to
age or sex. Anti-HCV was detected in the serum of 3 individuals (2.3 %). No differences among
age, sex or ethnicity regarding anti-HCV prevalence were found. The study group concluded that,
HBV vaccination programs will be necessary [23].
A study conducted by Subramanian K, et al, in Australia to determine Hepatitis B status in
refugees, increasing health burden in Western Australia. From a total of 478 with the majority
migrated from Asia (57%) and Africa (35%). About 50% of CHB patients are at risk of cirrhosis
and hepato- cellular carcinoma that do not get treatment. The study determines the prevalence of
Asian and African immigrants 0.05%. The investigators conclude that, increasing economic
burden of CHB patients and increasing direct costs of treatment [24].

8
Chloe J H, et al, conducted a cross-sectional study in USA to determine Hepatitis B and Liver
Cancer Beliefs among Korean Immigrants in Western Washington. The investigators select 30
participant interviews and belief that, food is main cause of hepatitis B transmission. Some of them
recognized by clinicians about HBV transition such as blood exposure, sexual contact, or
maternal–child vertical transmission (no interviews).The majority believe that prevent by altering
eating habits, avoiding contaminated meats. The investigators suggest that, vaccination will likely
require careful attention for misconception of transmission of HBV [25].
Another study performed in USA by Rein B D, et al, to determine the Prevalence of Hepatitis B
Surface antigen among refugees entering the United States Between 2006 and 2008.Refugees
screened from 20 areas a total of 42,303 refugees. The study indicated that highest HBsAg
prevalence from Africa (8.1%), Asia (4.8%) eastern Europe (2.6%), and South/Central America
and the Caribbean (1.0%).In Africa, the highest prevalence was observed in refugees from Eritrea
(15.5%); the lowest prevalence Burundi (3.0%).In Asia the highest prevalence from Myanmar
(12.4%).Prevalence in European countries ranged from 0.08%in Russia to 5.9% in Moldova.
Refugees from South American, Central American and Caribbean, prevalence below 2.0%, Haitian
refugees, and prevalence were 2.6%.The assessor concludes that, refugee prevalence may differ
from the prevalence among the general population [26].
In Northern California, a cross- sectional survey study was conducted by Levy V, et al, about
1,512 immigrant men aged 18 to 35 screened HBV prevalence and risk behaviors. Asian
immigrants have had prior HBV infection (15.1%) and chronic infection (3.8%) compared to US
born (prior 5.1%, chronic 0.6%) and Latino immigrant men (prior 2.0%, chronic 0.3%).The study
group concludes that, HBV testing and vaccination of immigrants soon after US arrival should be
encouraged [27].
The study conducted by Shire A M, et al, in Somalia, to know the status of Viral Hepatitis Among
Somali Immigrants in Minnesota: Association of Hepatitis C With Hepato-cellular Carcinoma.
The study group recruited 99 males and 66 females for anti-HCV from which 68 of 73 Somalis
(93.2%) with positive anti-HCV test results had active HCV infection. Of 30 Somali patients with
HCC, 22 (73.3%) tested anti-HCV positive viral hepatitis was diagnosed coincident with HCC.
The investigators concluded that, screening immigrants for HCV infection may enhance the
prevention, early detection, and optimal treatment of HCC [28].

9
A study performed by Cella E, et al, in 2016 to identify epidemiological analysis of Hepatitis B
virus infection in migrants. The study group recruited 136 Malian participants screened, HBV
positive 16 (11.7%),Hepatitis B serologic test results 13(81.25%) reactive for HBsAg and none for
HBs-Abs. Additionally HBeAg was reactive 11(68.75%).HCV-Ab-positivity 18.75%, all HCV-
RNA negative. The study group conclude that, give an important improvement in prevention
campaigns and monitoring of the viral infection in migrants. [29].
The study conducted by Daw M.A.et al,in Libia.2016 to assess; Geographic integration of hepatitis
C virus. A global threat prevalence of HCV in the world (14.7%-32%). It is alarming that > 20%
of Egyptian blood donors are seropositive for HCV. Libya, considered an area of low endemicity
for hepatitis C (1.2% average prevalence) In Iran, the prevalence of anti-HCV antibodies ranges
from 0.2% to 6.25% . HCV prevalence was higher in Iraq (2.3%), Jordan (3.5%) and the Gaza
strip (2.2%) Syria (1%).There is no national studies on the prevalence HCV in. The assessor
concludes that, geographic integration of HCV is reflected in the prevention and treatment of this
ongoing pandemic [30].
Short report presented by Franco-Paredes C, et al, in USA on untreated tropical infectious diseases
among Sudanese refugees in the United States. The reporters during the study period from July
2005 to December 2006,medical evaluations of the 44 of 150 Atlanta area lost boys,
mean age 25 years were completed. Of the 31 patients in whom we were able to obtain hepatitis B
diagnostic serologies, 10 (32%) showed evidence of HBsAg[31].
The study conducted by Chandrasekhar E, et al, in Chicago to identify of African-Born People
With Chronic Hepatitis B Virus infection in the Chicago Metropolitan Area, 2012–2014.The study
group selected 1,000 African-born people. Of which are Democratic Republic of the Congo
(14%), Nigeria (13%), Ghana (11%), Somalia (11%), and Ethiopia (10%). Of which 35 (8%)
HBsAg-positive people, 37% had evidence of past infection, and29% were immune. The study
group concludes that, the large proportion of HBsAg-positive people reinforces the need for health
promotion programs [32].

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3. Objectives

3.1. General Objective

To determine the Prevalence of Hepatitis B and C Viruses, Associated Risk Factors and
Knowledge, Attitude and Practice Among Refugees at Pugnido-I refugee camp in Gambela,
Ethiopia.

3.2. Specific objective

 To determine prevalence of hepatitis B and C viruses among refugees


 To assess associated risk factors related to Hepatitis B and C Viral infections in refugees
 To assess knowledge, attitude and practice among refugees about Hepatitis B and C Viral
infections

11
4. Hypothesis

Null hypothesis (HO)

The Prevalence of HBV and HCV in this study group is not different from in the previous studies
in Minnesota on Somalia migrants [28].

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5. Materials and Methods

5.1. Study design and period

A cross-sectional study was conducted to determine the prevalence of HBV and HCV by taking
blood samples and screened sera with rapid test and positive tests were further tested with ELISA,
and associated risk factors as well as KAP was assessed using a semi-structured questionnaire. The
study was conducted from January, 2018 to May, 2018 at Pugnido-I refugee camp in Gambella,
Ethiopia.

5.2. Study area


Gambela is the region that situated in South-West part of Ethiopia and borders with Benishangul
Gumuz and Oromiya regions to the North, the Southern Nations, Nationalities and Peoples’
Regional State (SNNPRS) and the South-Sudan Republic to the South, Oromiya and SNNPRS to
the east and the South-Sudan Republic to the west. Gambella is located to the southern direction
and apart about 711.2 km from Addis Ababa. In the region there are six refugee camps which
encompass the total of 285,846 refugees, namely Pugnido-II, 16, 820, Nguenyyiel 28,243, Kule
51,272, Jewi 56,989, Pugnido-I accounts about 62,925 and Tierkidi 69,597 refugees. Of which the
study was conducted at Pugnido-I refugee camp.

5.3. Population

5.3.1. Source of population

All refugees who were living at Pugnido-I camp during the study period.

5.3.2. Study population


Refugees who have living at Pugnido-I camp and visiting the refugees camp health center
during the study period and who were volunteer to participate in the study.

5.4. Inclusion and exclusion criteria

5.4.1. Inclusion criteria


Refugees aged ≥18 years.

5.4.2. Exclusion criteria


Refugees who knew their status of HBV and HCV.

13
5.5. Study variables

5.5.1 Dependent variables


 Prevalence of hepatitis B virus among refugees
 Prevalence of hepatitis C virus among refugees
 Knowledge, attitude practice (KAP) of refugees about HBV and HCV.

5.5.2. Independent variables


 Socio demographic (Sex, age, marital status, educational status)
 History of multi sexual partner in life
 Sharing of sharp materials
 History of tattooing
 Family history of liver disease
 History of tooth extraction
 HBV vaccination status
 Awareness of hepatitis/liver disease/
 Sexual transmission of hepatitis infection
 Body fluid transmission of hepatitis infection
 HBV have vaccine

14
5.6. Sample size and sampling procedure

5.6.1 Sample size determination


The estimated sample size was about 384 participants assuming a proportion of 50%.Sample size
derived using the following formula:

n = ( Zα/2)2 x p (1-p)
d2

Where: n= sample size; Zα/2 = standard normal distribution abscissa corresponding to


95% confidence interval (1.96); P = proportion of 50%, Q = (1-P); and d = desired level of
precision (5%).

n = (1.96)2 x 0.5(1-0.5 )=384

(0.05)2

For the calculation, a 95% confidence interval and a 5% margin of error is used. To minimize
errors arising from the likelihood of non-compliance/non response/, ten percent (10%) of the
sample size is added giving a final sample size of 422.However, we have collected 453 samples.

5.6.2. Sampling Technique

Purposive sampling technique was used to select refugee camps due to well organized laboratory,
huge number of refugees in the camp and convenient sampling technique was used to select study
participants who visited the clinic during the study period.

5.7. Data collection and laboratory Analysis

5.7.1. Data collection

Written consent was obtained from study groups and after that questionnaire was used to collect
informa.tion about knowledge, attitude and practice of the disease, the exposure status of potential
risk factors and to assess the socio demographic characteristics of the study participants was used.

15
The questionnaire was prepared in English language by principal investigator in simple
understandable language. Information was given to the study participants about; the benefit of the
study, individual’s right, informed consent and before started the data collection

5.7.2. Laboratory analysis


After obtaining the participant written consent, 5ml of blood sample was collected from each
refugee using gel and clot activator tubes. The tubes were label and process at the time of
collection. The blood sample was centrifuge for 10 minutes at speed of 3000rpm and the serum
was separated. After separation, all serum samples were tested for HBsAg with rapid screening
method according to the manufacturer’s instruction of the selected test kit then, all serum samples
were transported using cold box to Ethiopian Airports Enterprise clinic laboratory and anti-HCV
rapid screening was performed. All rapid positive tests were confirmed using ELIASA at Ethiopian
Public Health Institute (EPHI). All serum samples which tested positive by rapid test for HBsAg
and anti-HCV were further tested with ELISA for confirmation.

5.7.2.1. HBsAg rapid test principle


The principle of the test is immune-chromatography which has two unique site immune-assays on

a membrane. The test sample flows through the membrane assembly of the cassette, the color

monoclonal anti-HBsAg, colloidal gold conjugate complexes with HBsAg in the sample. This

complex moves further on the membrane to the test region where it is immobilized by another

monoclonal anti-HBsAg antiserum coated on the membrane. Pink-purple color band formation

confirms a positive test result and absence of the color band in the test region indicates a negative

test result. Un reacted conjugate and unbound complex, if any moves further on the membrane and

are subsequently immobilize by the anti-rabbit antibodies coated on the membrane at the control

region, forming a pink/purple color band. This control band serves to validate the test result (Test

kit insert sheet).

16
5.7.2.2. Anti-HCV rapid test principle
Rapid test which is followed the principle of immune-chromatography, unique two site
immunoassay on a membrane. As the sample flows through the membrane of the test cassette, the
test color HCV antibody colloidal gold conjugate complexes with anti-HCV in the sample. This
complex moves further on the membrane to the test region where it is immobilized by HCV
antigen coated on the membrane leading to formation of a pink-purple color band which confirms
a positive test result. Absence of this color band in the test region indicates a negative test result.
Un reacted conjugate and unbound complexes, if any moves further on the membrane and are
subsequently immobilize by the anti-HCV coated on the membrane at the control region, forming
a pink/purple color band. This control band serves to validate the test result (Test kit insert sheet).

5.7.2.3. HBsAg ELISA test principle


This is a Sandwich Enzyme linked Immune-sorbent assay method in which polystyrene micro-
well strips are pre-coated with monoclonal antibodies specific to HBsAg. Participants serum or
plasma sample is added to the micro-wells together with a secondary antibody conjugated with
horseradish peroxidase (HRP) and directed against a different epitope of HBsAg. During
incubation, the specific immune-complex formed in the case of presence of HBsAg in the sample,
is captured on the solid phase. After washing to remove sample serum protein and unbound HRP-
conjugate, chromogen solution containing Tetra-methyl Benzedrine (TMB) and urea peroxidase
are added to the walls. In the presence of the antibody-antigen-antibody (HRP) sandwich immune-
complex, the colorless chromogens are hydrolyzed by the bound HPR conjugate a blue colored
product. The blue color turns to yellow after stopping the reaction with sulfuric acid. The amount
of color can be measured and is proportional to the amount of antigen in the sample (Test kit insert
sheet).

5.7.2.4. Anti-HCV ELISA test principle


Polystyrene micro-well stripes are pre-coated with recombinant, highly immune-reactive antigens
corresponding to the core and non-structural regions of HCV. During the first incubation step, anti-
HCV specific antibodies, if present, will be bound to the phase pre-coated HCV antigens. The
wells are washed to remove unbound serum proteins, and rabbit antihuman IgG antibodies (anti-
IgG) conjugated to HRP is added. During the second incubation step, these HRP conjugated
antibodies will be bound to any antigen- antibodies complexes previously formed and the unbound

17
HRP-conjugate is then removed by washing. Chromogen solutions containing Tetra-methyl
Benzedrine (TMB) and urea peroxidase are added to the wells and in presence of the antigen-
antibody-anti-IgG (HRP) immune-complex; the colorless chromogens are hydrolyzed by the
bound HRP-conjugated to a blue colored product. The blue color turns to yellow after stopping the
reaction with sulfuric acid. The amount of color can be measured and is proportional to the amount
of antibody in the sample.

5.8. Data entry and analysis


The coded data was entered and analyzed by SPSS software version 20. In the analysis process,
frequency distributions of variables were workout in order to describe in relation with the study
population. Descriptive statistics like, percentage and ratio were calculated. The associations
between dependent and independent variables were measured by means of odds ratio for which
95% confidence interval was calculated. Variable that show a statistically significant association
(p<0.05) was analyzed at bivariate and multivariate level.

5.8.1. Quality assurance and quality control

The quality of data was controlled starting from the time of questionnaires preparations. The
questionnaires were developed by reviewing relevant literatures on the subject to ensure reliability.
Instruction was given for data collectors on the purpose of study and procedures of data collection
before started the study. During data collection, the principal investigator was receiving
questionnaires from data collectors and review for completeness, accuracy, and consistency.
Standard operating procedure (SOPs) of tests was followed during laboratory analysis and a known
positive and negative serum for HBV and HCV testing was used. The result was entering to
statistical software to analyze and summarize the data.

5.9. Ethical considerations

An ethical review committee of the Department of Clinical Laboratory Sciences, School of Allied
Health Sciences, College of Health Science, and Addis Ababa University was approved this study
with an ethical letter. After written permission was obtain from the office of the Administration of
Refugees and Returnees Affair and UNHCR. Names and any other sensitive personal information
of individual study subject was not record during sample collection. Moreover the sample

18
collectors were laboratory professional working in the laboratory department of the refugee clinic
and were being monitored daily by the principal investigator. Sample was collected after getting
consent from the participant refugees. All positive results were communicated to the attending
physician. The confidentiality of the test result of the study was kept by investigator.

5.10. The overall work flow diagram

19
Site assessment and select refugee camps.

Pugnido-I refugee camp was selected based on the laboratory facility and
duration of the camp as well as the number of refugees which is 62,925.

Ethical review letter from SLS and permission letter from ARRA office obtained.

Consent was obtained from study participants. Socio-demographic, associated risk factors and
KAPs related data was gathered.

Venous Blood was draw from participant and serum was separated

ELISA was done for


HBsAg Rapid test was Anti-HCV Rapid test was confirmatory
performed test both HBsAg and HCV
performed

Fig-1 .Work flow diagram of the study

20
5.11. Operational definitions
Refugees: South Sudan immigrants live in pugnido-I camp in Gambella
HBV positive: Serum positive for HBsAg by rapid test and ELISA method
HCV Positive: Serum positive for anti-HCV by rapid test and ELISA method
HBsAg: low (<2%), intermediate (2–8%), and high (>8%) according to WHO [4].

21
6. Results

6.1: Socio-Demographic Characteristics

During the study 473 volunteer clinic visitors have given their consent to be participating in the
study and the questionnaire was filled, but 11 participants were excluded due to improper blood
collection and 9 participants were rejected with incompleteness of the questionnaire with the total
rejection of 4.2% (n=20/473). From the total of 453 participants 81.7 %(n=370/453) were female
and 18.3%(n=83/453) were male and the age range of the participants 18-61years old and the mean
age was 29.6±9.3SD. Majority of age group was 26-35, 43.3 %( n=196/453). Related to marital
status and educational status, 83.7 %( n=379/453) of them were married and 36.6 %( n=166/453)
participants were elementary level respectively as showed in (Table 6.1).
Table 6.1: Socio-Demographic Characteristics among refugees of Pugnido-I camp Gambela,
Ethiopia, January to May 2018 (n=453), 2018.
Variables Frequency(n=453) Percentage (%)
Sex Female 370 81.7
Male 83 18.3
Age category 18-25 167 36.9
26-35 196 43.3
36-45 57 12.6
46-55 24 5.3
>55 9 2.0
Marital status Single 25 5.5
Married 379 83.7
Divorced 22 4.9
Widowed 27 6.0
Education Illiterate 165 36.4
Elementary 166 36.6
High school 104 23.0
Higher education 18 4.0
n=total sample size

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6.2. Prevalence of HBV and HCV
All participants were screened with HBsAg and Anti-HCV rapid tests. From those 7.3 %(
n=33/453) were positive for HBsAg and 2.2 %( n=10/453) were positive for Anti-HCV. ELISA
confirmed prevalence of HBV and HCV among refugees was 7.3 %(n= 33/453) and2.0 %(
n=9/453) respectively. Of those 6.8% (n=25/370) and 1.4% (n=5/370) of females were positive
for HBV and HCV respectively. And 9.6 % (n=8/83) and 4.8 % (n=4/83) of males were positive
for HBV and HCV respectively. In the case of Age category, 36-45years old 12.3 %( n= 7/57)
were positive for HBV which is slightly higher than other age categories. Participants who were
positive for HBV 7.7 %( n= 29/379) and 2.4 %( n=9/379) positive for HCV were married. In the
case of educational status 12.0% (n=20/166) for HBV positive and 3.0% (n=5/166) for HCV
positive refugees were educated at elementary level (Table 6.2).
Table 6.2: Prevalence of HBV and HCV among refugees of Pugnido-I camp Gambela
Ethiopia January to May 2018 (n=453), 2018.
Variables HBsAg ELISA Anti-HCVELISA Total

Pos (%) Neg(%) Pos (%) Neg(%)


Sex Female 25(6.8) 345(93.2) 5(1.4) 365(98.6) 370
Male 8(9.6) 75(90.4) 4(4.8) 79(95.2) 83
Age category 18-25 7(4.2) 160(95.8) 2(1.2) 165(98.8) 167
26-35 17(8.7) 179(91.3) 2(1.0) 194(99.0) 196
36-45 7(12.3) 50(87.7) 2(3.5) 55(96.5) 57
46-55 2(8.3) 22(91.7) 1(4.2) 23(95.8) 24
>55 0(0) 9(100) 2(22.2) 7(77.8) 9
Marital status Single 1(4.0) 24(96.0) 0(0) 25(100) 25
Married 29(7.7) 350(92.3) 9(2.4) 370(97.6) 379
Divorced 1(4.5) 21(95.5) 0(0) 22(100) 22
Widowed 2(7.4) 25(92.6) 0(0) 27(100) 27
Educational status Illiterate 7(4.2) 158(95.8) 4(2.4) 161(97.6) 165
Elementary 20(12.0) 146(88.0) 5(3.0) 161(97.0) 166
High school 5(4.8) 99(95.2) 0(0) 104(100) 104
Higher education 1(5.6) 17(94.4) 0(0) 18(100) 18
Total 33(7.3) 420(92.7) 9(2.0) 444(98.0) 453
HBsAg-hepatitis B surface antigen,ELISA-Enzyme Linked Immunoassay,HCV-Hepatiti C virus.

23
6.3: Risk factors associated with prevalence of HBV
Among female participants 6.8% (n=25/370) were positive for HBV and 9.6% (n=8/83) of males,
the difference was not statistically significant (COR=0.679, CI 95%=0.295-1.565,
P=0.364).Among participants 7.7%(n=29/379) were married (COR=1.989, CI95%=0.26015.231,
P=0.508), 1.4%(n=1/22) were divorced,7.4%(n=2/27) were widowed, and 4.0% (n=1/25) were
single, there was no statistically significant difference between marital status and hepatitis virus
infection. Regarding to educational status, those who were elementary level were 12.0 %(n=
20/166)positive for HBV but there was no statistically significant difference between educational
status and HBV positivity(COR=2.329,CI95%=0.294-18.459,P=0.424).Participants who have
exchange of sharp materials with other person have slightly higher positivity of HBV 6.3%
(n=12/106), however there was no statistically significant difference between associated risk
factors HBV reactivity(COR=0.828,CI 95%=0.281-2.438,P=0.731) as showed in (Table 6.3).

24
Table 6.3: Risk Factors associated with prevalence of HBV based on ELISA test among
refugees of Pugnido-I camp Gambela, Ethiopia (n=453), 2018.
Variables No(%) HBsAg pos=no (%) COR CI (95%) P- Value
Sex Female 370(81.7) 25(6.8%) 0.679 0.295-1.565 0.364
Male 83(18.3) 8(9.6%) 1

Age category * 18-25 167(36.9) 7(4.2)


26-35 196(43.3) 17(8.7)
36-45 57(12.6) 7(12.3)
46-55 24(5.3) 2(8.3)
>55 9(2.0) 0(0)
Marital status Single 25(5.5) 1(4.0) 1
Married 379(83.7) 29(7.7) 1.989 0.260-15.231 0.508
Divorced 22(4.9) 1(4.5) 1.143 0.067-19.424 0.926
Widowed 27(6.0) 2(7.4) 1.920 0.163-22.584 0.604
Education status Illiterate 165(36.4) 7(4.2) 0.753 0.087-6.493 0.796
Elementary 166(36.6) 20(12.0) 2.329 0.294-18.459 0.424
High school 104(23.0) 5(4.8) 0.859 0.094-7.810 0.892
Higher 18(4.0) 1(5.6) 1
education
Multi sex Yes 347(76.6) 21(6.1) 0.505 0.239-1.063 0.072
No 106(23.4) 12(11.3) 1
Sharps Yes 64(14.1) 4(6.3) 0.828 0.281-2.438 0.731
No 389(85.9) 29(7.5) 1
Tattoo Yes 18(4.0) 1(5.6) 0.741 0.095-5.747 0.774
No 435(96.0) 32(3.4) 1
Family liver* Yes 8(1.8) 0(0.0)
No 445(98.2) 33(7.4)
Tooth extract Yes 51(11.3) 3(5.9) 0.775 0.228-2.636 0.683
No 402(88.7) 30(7.5) 1
Vaccine Yes 9(2.0) 1(1.1) 1.609 0.195-13.271 0.658
No 444(98.0) 32(7.2) 1
Family liver history*, Age category *, not valid for association, COR-Crude odds ratio.

25
6.4. Risk Factors associated with HCV prevalence

Among female and male participants 1.4 % (n= 5/370) and 4.8% (n=4/83) were positive for HCV
respectively, the difference was not statistically significant (COR= 0.271, CI 95%=0.071
1.030,P=0.055). Statistically significant association was showed on the age group of 18-25 and
26-35 years old with HCV positivity (COR=0.042, CI 95%=.0.005-0.374, P=0.003 and
COR=0.036, CI 95%=0.004-0.295, P=0.002, respectively). Association was not performed for
marital status and educational status. Among participants 1.6 %( 1/64) have sharing of sharp
materials; however there was no significant association between exchange of sharp materials and
HCV positivity as demonstrated in (Table 6.4).

26
Table.6.4. Risk Factors associated with prevalence of HCV based on ELISA test among
refugees at Pugnido-I camp Gambela Ethiopia January to May 2018 (n=453), 2018.
Variables No (%) Anti-HCV COR CI (95%) P- Value
Pos
Sex Female 370(81.7) 5(1.4) 0.271 0.071-1.030 0.055
Male 83(18.3) 4(4.8) 1
Age category 18-25 167(36.9) 2(1.2) 0.042 0.005-0.374 0.003
26-35 196(43.3) 2(1.0) 0.036 0.004-0.295 0.002
36-45 57(12.6) 2(3.5) 0.127 0.015-1.052 0.056
46-55 24(5.3) 1(4.2) 0.152 0.012-1.940 0.147
>55 9(2.0) 2(22.2) 1
Marital status* Single 25(5.5) 0(0)
Married 379(83.7) 9(2.4)
Divorced 22(4.9) 0(0)
Widowed 27(6.0) 0(0)
Education status* Illiterate 165(36.4) 4(2.4)
Elementary 166(36.6) 5(3.0)
High school 104(23.0) 0(0)
Higher education 18(4.0) 0(0)
Multi sex history Yes 347(76.6) 7(2.0) 1.071 0.219-5.233 0.933
No 106(23.4) 2(1.9) 1
Sharps material Yes 64(14.1) 1(1.6) 0.756 0.093-6.148 0.794
No 389(85.9) 8(2.1) 1
Tattoo history* Yes 18(4.0) 0(0.0)
No 435(96.0) 9(2.1)
Family liver* Yes 8(1.8) 0(0.0)
No 445(98.2) 9(2.0)
Tooth extract* Yes 51(11.3) 0(0.0)
No 402(88.7) 9(2.2)
HBV Vaccine * Yes 9(2.0) 0(0.0)
No 444(98.0) 9(2.0)
Variables marked with*: not valid for association, CI-Confident interval COR-Crude odds ratio,

27
6.5. Adjusted Odds Ratio of sex and age with prevalence of HCV
Adjusted odds ratio was performed between Sex and age with HCV and showed statistically
significant association as follows: Sex (AOR=0.291,CI=O.072-1.177,P=0.083) age category of
18-25 years (AOR=0.045,CI=0.005-0.378,P=0.004) age category of 26-35 years
(AOR=0.035,CI=0.004-0.301,P=0.002) and age category of 36-45 years (AOR=0.111,CI=0.013-
0.974,P=0.047 (Table 6.5).These the above age categories were slightly less associated to HCV
infection.
Table 6.5.Adjusted odds ratio for age and sex with HCV infection based on ELISA test
among refugees at Pugnido-I camp Gambela Ethiopia January to May 2018 (n=453), 2018.
Variables No (%) Anti –HCV AOR CI (95%) P-Value
Positive
Sex Female 370(81.7) 5(1.4) 0.291 0.072-1.177 0.083
Male 83(18.3) 4(4.8) 1
Age 18-25 167(36.9) 2(1.2) 0.045 0.005-0.378 0.004
category
26-35 196(43.3) 2(1.0) 0.035 0.004-0.301 0.002
36-45 57(12.6) 2(3.5) 0.111 0.013-0.974 0.047
46-55 24(5.3) 1(4.2) 0.136 0.010-1.827 0.132
>55 9(2.0) 2(22.2) 1

AOR= Adjusted odds ratio


CI = Confidence interval

28
6.6. Knowledge, Attitude and Practices (KAP) assessment on HBV and HCV
6.6.1. Knowledge of participants

Majority of participants 79.2% (n=359/453) were never heard about HBV and HCV and 86.5%
(n=392/453) and 91.4% (414/453) were never know the transmission of HBV and HCV. About
89.0 % (n=403/453) participants have no ideas about liver cancer with the causative agent of HBV
and HCV. In case of vaccine 86.8% (n=393/453) do not have information about availability of
HBV vaccine and 72.0% (n=326/453) also not know the treatment of HBV and HCV at all (Table
6.6).
6.6.2. Attitude of participants
In this study 8.2 %(n=37/453) refugees believed that HBV and HCV can transmit through food
and 11.5% (n=52/453) participants were believed that HBV and HCV are curable diseases. About
75.7% (n=343/453) participants were believe that HBV and HCV is not serious public health
problems and 72.8% (n=330/453) participants were believed that vaccine of HBV is not safe(Table
6.6).
6.6.3. Practice of participants
With regard to vaccination, 98.5% (n=446/453) were not vaccinated to HBV. Screening of HBV
and HCV, 87.2% (n=395/453) were not screened, 99.8% (n=452/453) of refugees did not have
practice of exchange of injection drugs (Table 6.6).

29
Table 6.6.Knowledge, Attitude and Practice assessment on HBV and HCV among refugees
at Pugnido-I camp Gambela, Ethiopia, January to May 2018 (N=453), 2018.

Knowledge assessment questions (n=453) (n=453)


Yes (%) No (%)
Have you ever heard about HBV and HCV infection? 94(20.8) 359(79.2)
Is Hepatitis transmitted through sex? 61(13.5) 392(86.5)
Can you get hepatitis infection through body fluid contact? 39(8.6) 414(91.4)
Do HBV and HCV cause liver cancer? 50(11.0) 403(89.0)
Does HBV have vaccine? 60(13.2) 393(86.8)
Is there effective treatment for HBV and HCV? 127(28.0) 326(72.0)
Attitude assessment questions
Do you believe HBV &HCV transmitted through food? 37(8.2) 416(91.8)
Do you think hepatitis infection is curable disease? 52(11.5) 401(88.5)
Do you believe hepatitis infection is serious public health 110(24.3) 343(75.7)
problem?
Do you think taking HBV vaccine is safe? 123(27.2) 330(72.8)
Practice assessment questions
Have you received HBV vaccination? 7(1.5) 446(98.5)
Have you screened for HBV and HVC? 58(12.8) 395(87.2)
Have you exchange of injection drug uses 1(0.2) 452(99.8)

HBV-Hepatitis B Virus, HCV-Hepatitis C virus.

30
7. Discussions
Hepatitis viral infection due to HBV and HCV are widespread infectious diseases representing
major health problems. It is well known that refugees constitute a special social group in a
geographical area in which, they often live under conditions that facilitate the spread of infectious
diseases [11].

The prevalence of HBV among refugees in this study was 7.3%(n=33/453) which was a lower
finding compared to previous studies done in different African migrants those done in different
countries. In Mali (11.7%)[28], in USA African migrants: Eritrea(15.5%), Ethiopia(9.1%),
Somalia(8.3%)[26]. This finding was also a lower finding compared to studies done in different
parts of the World immigrants such as: In Bari-Italy (8.3 %)[3], in Athens (15.4 %)[11],in South-
Europe(11.9%)[12], in Pakistan-Afghan refugees (8.3%)[14], in India-Tibetan
refugees(8.9%)[15],in Naples-Italy immigrants from different origin of countries such as; Eastern-
Europe(15.7%),Asia(27.3%),Cambodia(8%) Albania (11.7%), Vietnam(9.3%)[19],in South-
Italy(9.6%)[20],in Italy(10.7%)[21],in Athens (15.4%)[23], in Chicago(8.0%)[32].This might be
because our study populations are all volunteer refugees and most of them could be confident of
their sero-status, and difference in the study period, study subjects, sample size, might also be the
cause of such differences.

In differently to the above comparison the prevalence of HBV in the current study was also higher
than studies in USA African migrants such as: Ruanda (5.9%),Kenya(4.1%),Tanzania
(3.1%0),Burundi(3.0%),Sudan(6.8%)[26].Around the World; in UK(5.0 %)[6], Canada (3.0%)[9],
Malta(0.68%), India (6.2%) [10],NW-Europe(3.8%)[13],Kosovo (2.9%)[17],in Italy China-
migrants (6.0%),Turkey-migrants (5.0%)[19].The differences might be due to variations in
geographical distribution as well as population differences in terms of lifestyle, awareness.

HCV prevalence in the present study was 2.0 % and our finding was lower than the studies done
in different refugees; for instance; in Bari-Italy(4.5%)[3],in Canada(3.0%)[9],in Athens
(2.3%)[11],in Izmir(4.5%)[7] in Roma (23.4%) [2],in Spain(3.1%)[2],in Albania(2.3%)[2],in Sub-
Saharan Africa(2.2%)[2].This study finding on HCV prevalence was higher than previous studies
from Netherlands (1.5%)[2], Kosovo(0.7%) [2],Turkey(0.1%) [2],Malta(0.6%) [10], Germany

31
(1.9%) [22]. This difference might be due to difference in geographical location and sample size
of participants.
Among female participants 6.8% (n=25/370) were positive for HBV and 9.6% (n=8/83) were
males, however, the difference was not statistically significant (COR=0.679, CI 95%=0.295-1.565,
P=0.364). From the total of female participants 1.4% (n=5/370) were positive for anti-HCV and
4.8 %(n=4/83) males were positive for anti-HCV but the difference was not statistically significant
(COR= 0.271, CI 95%=0.071 1.030,P=0.055).This finding was incomparable to a study conducted
in Barry Italy from the total of 442 male participants 9.7% (n=43/442) were positive for HBsAg
and from the total of 87 female 1.1% (n=1/87) were positive for HBsAg where as
48.4%(n=214/442) males were positive for anti-HCV and 31%(n=27/87) females were positive
for HCV [3]. The difference might be due to sex proportion and sample size.
In relation to marital status, prevalence of HBV was higher among married participants, which
was 6.4 %( n= 29/453) but the difference was not statistically significant (P>0.05),in Pakistan
15.6% (58/903) was married higher than our study[14].Regards to education refugees who were
elementary level were 4.4 %( 20/453) positive for HBV but there was no statistically significant
difference between educational status and HBV positivity(P>0.05).In Cebu, Philippine2% (9/450)
was elementary level[36].And also Participants who have exchange of sharp materials with other
person were 11.3% (12/106) positivity, however there was no statistically significant difference
between associated risk factors HBV reactivity(P>0.05)[15].
The age group 36-45 was highly prevalence of HCV which was 12.3% (n=7/57).The study showed
that Age group 18-25 was prevalence 1.2% for HCV and 26-35 was prevalence 1.0% for HCV and
statistically significant with HCV positivity which was (P=0.003 and P=0.002) respectively. The study
conducted in Minnesota the same age group prevalence was HCV 5.4 %( n= 48/883) was higher than our
study [28].
This study also assessed the knowledge, attitudes and practices of participants towards to HBV
and HCV infection. Majority of participants for instance 79.2% (n=359/453) were responded that
they have never heard about HBV infection in other ways they had low knowledge of hepatitis
infection. The study in Cebu, Philippine (84%) the study participants replied that they do not have
knowledge in terms of: hepatitis B and C viral diseases [36]. In terms of mode of transmission
86.5% (n=392/453) and 91.4% (n=414/453) were never know how the HBV and HCV infection
transmitted through sex and body fluid respectively. In Cebu, Philippine (78%), that the diseases

32
could be transmitted by unsafe sex [36].In case of vaccine 86.8% (393/453) participants did not
have information about availability of HBV vaccine, in Philippine (90%) participants answered
that there is a vaccination available for these diseases[36]. The above data showed that all most all
the majority of participants have limited knowledge about HBV and HCV infection, transmission
and protection. Therefore, the magnitude of HBV and HCV will be increased in the refugees as
well as in the local society unless we have making awareness with formulating health education
program in the refugees and as the same time in the local society.
With regard to participants attitude, 8.2 %( n=37/453) were believe that HBV and HCV can
transmit through food, in Western Washington Participants expressed that the contamination of
food sources and the sharing of used utensils were the most significant sources of hepatitis B
transmission [25]; about 72.8% (n=330/453) participants believed that vaccine of HBV is not safe
which is in line with study in Philippine (72%)[36].
In relation to participants practice, screening and vaccination of HBV and HCV was assessed using
questions of which 87.2% (n=395/453) responded not screened and 98.5% (n=446/453) were not
vaccinated respectively. In Philippine majority of the respondents did not do screening for hepatitis
B or C (94%)[36].In Ethiopia the study performed by different group the overall prevalence of
hepatitis B virus (HBV) was 7.4%,in community based studies 8.0% in blood donors, 8.4%[37]
which was higher than our study result(7.3%). The difference might be due to large sample size
in their study and different target group. Anti -HCV prevalence conducted in kemissie and Omo
at community level which was 1.3%, this was lower than our finding (2.0%) [37].The difference
might be due to high risk target group in our study.

33
8. Strength and Limitation of the study

8.1. Strength of the study


 The research is conducted for the first time.
 The research was performed among high risk groups

8.2 Limitation of the Study

 Unable to perform all hepatitis panels


 We did ELISA only for those sera which were positive by rapid tests

34
9. Conclusion and Recommendation

9.1. Conclusion
In general the prevalence of hepatitis B and C viruses was intermediate in Gambela refugee
camp. The age category of 18-25, 26-35 and 36-45 years had significant association with
hepatitis C infection. Majority of the participants had limited knowledge about the
transmission and protection of HBV and HCV infection. There was no significant association
between proposed risk factors and hepatitis B and hepatitis C.

9.2. Recommendations

 National surveillance screening for Hepatitis B and C among Ethiopian refugees is


required.
 Conducting regular health education for refugees and the local population to prevent the
transmission of hepatitis.
 Formulate the screening policy of HBV and HCV among refugees especially urban
refugees is vital.
 Large scale study is important to make generalization among refugee in Ethiopia.

35
10. References
1. CDC, Viral hepatitis Surveillance United States, 2011, availablehttps://www.cdc.gov/accessed
7 Oct 2017

2. European Center for Disease Prevention and Control, technical report; Hepatitis B and C in
the neighborhood: prevalence, burden of disease and screening policies, 2010,available at
www.ecdc.europa.eu, accessed 17 Oct 2017.
3. Tafuri S, Prato R, Martinelli D, Melpignano L, Palma M D, Quarto M, et al. Prevalence of
Hepatitis B and C viruses, HIV and syphilis markers among refugees in Bari, Italy; BMC
Infectious Disease 2010,10:213.1-5.
4. WHO, Guideline on hepatitis B and C tests, February 2017, available at
https://www.finddx.org/wp-content/uploads/2017/02/WHO-guidelines-HBV-HCV-testing-
2017.accessed 7 Oct 2017
5. Hahné S J, Veldhuijzen I K, Wiessing L, Lim T, Salminen M, Laar M V. Infection with
hepatitis B and C virus in Europe:a systematic review of prevalence and cost effectiveness of
screening: BMC Infectious Diseases 2013, 13:181.
6. Evlampidou I, Hickman M, Irish C, Young N, Oliber I and Gillet S, et al. Low hepatitis B testing among
migrants: a cross-sectional study in UK city ;British J General Practice, 2016:1-10.
7. Kose S, Kuzucu L ,Gozaydın A, Yılmazer T. Prevalence of Hepatitis B and C Viruses Among
Asylum Seekers in Izmir; J I M H;2013:DOI 10.1007/s10903-013-9876-7: 1-3
8. Hayden T M, Deborah Lee D, Raeva L G, Drobeniuc J, Stauffer W M, Teshale E, Kamili S.
Hepatitis B Virus and Hepatitis C Virus Infections in United States-Bound Refugees from Asia
and Africa in Atlanta Georgia Am. J. Trop. Med. Hyg., 2014, 90(6): 1014–1020.
9. Greenaway C, Wong D K H, Assayag D, Deschenes M, Hui C, Ueffing E, et al. For the
Canadian Collaboration for Immigrant and Refugee Health; Guideline for immigrant health,
Screening for hepatitis C infection: evidence review for newly arriving immigrants and
refugees; CMAJ, 2011:1-14.
10. Padovese V, Egidi A M, Melillo T M, Farrugia B, Carabot P, Didero D,et al. Prevalence of
latent tuberculosis, syphilis, hepatitis B and C among asylum seekers in Malta; J P H 2013:
36(1) 22-27.

36
11. Roussos A, Goritsas C, Pappas T, Spanaki M, Papadaki P, Ferti A. Prevalence of hepatitis
B and C markers among refugees in Athens. World J Gast, 2003; 9(5):993- 995.
12.Katsanos K H, Resuli B F, Tsianos E V. Hepatitis B in Albanian refugees across Southeast
Europe: from epidemiology to vaccination and prevention policy; J A gastroenterology 2004,
17(2):160-167.
13. Chu J J, Wormann T, Popp J, Patzelt G, Akmatov M K, Kramer A, et al. Changing
epidemiology of Hepatitis B and migration a comparison of six Northern and North-Western
European countries;European Journal of Public Health, 2012, 23,(4), 642–647.
14.Quddus A, Luby S P, Jamal Z, Jafar T. Prevalence of hepatitis B among Afghan refugees
living in Baluchistan, Pakistan; Int J Inf ,2006:10, 242- 247.
15. Stevens K, Palmo T,Wangchuk T,Solomon S,Dierberg K and Hoffmann C J.HepatitisB
Prevalence and Treatment Needs Among Tibetan Refugees Residing in India; Jornal of
Medical Virology,2016, 88:1357–1363.
16. Hussein N R, Abdullah I M,Younus O M,Taher A,Salim A A and Shahab F I. Prevalence of
HBV, HCV and HIV Infections Among Syrian Refugees in Kurdistan Region, Iraq; Int J
Inf, 2017, 4(2):1-3.
17. Chironna M,Germinario C,Lopalco P L,Carrozzini F,Quarto M. Prevalence of Hepatitis Virus
Infections in Kosovar Refugees;Int J Infect Dis 2001; 5:209-213.
18. Owiti J A,Greenhalgh T,Sweeney L,Foster G R and BhuiK S. Illness perceptions and
explanatory models of viral hepatitis B & C among immigrants and refugees in UK; BMC
Public Health ,2015, 15:151.
19. Coppola N, AlessioL,Pisaturo M,Macera M,Sagnelli C,Zampino R, et al. Hepatitis B virus
infection in immigrant populations Naples,Italy; World J Hepatology,2015, 7(30).
20. Coppola N, Alessio L,Gualdieri L, Pisaturo M,Sagnelli C, Minichini C, et al. HepatitisB virus
infection in undocumented immigrants and refugees in Southern Italy: demographic,
virological, and clinical features; J Inf D Poverty ,2017, 6:33.
21. Palumbo E,Scotto G,Faleo G,Cibelli D C,Saracino A and Angarano G. Prevalence of HBV-
genotype in immigrants affected by HBV-related chronic active hepatitis in Italy, JArq
Gastroenterol, 2007, 44(1),54-57.
22. Greenaway C, Ma A T, Kloda L A, Klein M,Cnossen S,Schwarzer G, et al. The
Seroprevalence of Hepatitis C Antibodies in Immigrants and Refugees from Intermediate and

37
High Endemic Countries: A Systematic Review and Meta-Analysis in Germany; Journal
pone, 2015 10(11):1-19.
23. Roussos A,Goritsas C, Pappas T,Spanaki M, Papadaki P,Ferti A. Prevalence of hepatitis B
and C markers among refugees in Athens;World J Gastroenterol, 2003;9(5):993-995.
24. Subramaniam K, Flexman J, Tarquinio L, Thambiran A, Hopkins S and Cheng W. Hepatitis B
status in migrants and refugees: increasing health burden in Western Australia;Int M J; 2011;
880-886.
25. Choe J H, Chan N, Do H H, Woodall E, Lim E, Taylor V M. Hepatitis B and Liver Cancer
Beliefs among Korean Immigrants in Western Washington;JCS,2005,V 104(12):2955-2958.
26. Rein D B, Lesesne S B, Fallon A O, and Weinbaum C M. Prevalence of Hepatitis B Surface
Antigen among Refugees Entering the United States Between 2006and 2008; JHS, 2010;
51:431-434.
27. Levy V, Yuan J, Ruiz J,Morrow S, Reardon J, Facer M, et al. Hepatitis B Seroprevalence and
risk behaviors among immigrant men in a population-based household survey in low-income
neighborhoods of Northern California;J Immigrant Minority Health,2010,12:828–833.
28. Shire A M, Sandhu D S, Kaiya J K,Oseini A M,Yang J D,Chaiteerakij R,et al. Viral
Hepatitis Among Somali Immigrants: Association of Hepatitis C With Hepatocellular
Carcinoma in Minnesota;Mayo Clin Proc. 2012;87(1):17-24
29. Cella E, Ceccarelli G,Vita S, Lai A, Presti A. L, Blasi A, et al. First epidemiological and
phylogenetic analysis of Hepatitis B virus infection in migrants from Mali;Journal of Medical
Virology,2016,1-21.
30. Daw M A, El-Bouzedi A A, Ahmed M O, Dau A A, Agnan M M, Drah A.M. Geographic
integration of hepatitis C virus,a global threat, in Libiya; World J Virol2016,12; 5(4): 170-
182.
31. Franco-Paredes C, Dismukes R, Nicolls D, Hidron A,Workowski K,Morales A, et al. Short
Report: Persistent and Untreated Tropical Infectious Diseases Among Sudanese Refugees in
the United States, in Atlanta Georgia. Am. J. Trop. Med. Hyg., 77(4), 2007, 633–635.
32. Chandrasekar E, Song S, Johnson M, Harris A M, Kaufman G I, Freedman D, et al.A Novel
Strategy to Increase Identification of African-Born People With Chronic Hepatitis B Virus
Infection in the Chicago Metropolitan Area, 2012–2014;CDC.2016,13, 1-7.

38
33.Scott K C,Taylor E M, Mamo B,Herr N D,Cronkright P J,YunK,et al. Hepatitis B Screening
and Prevalence Among Resettled Refugees — United States, 2006–2011;MMWR / June 5,
2015 / 64 /21.
34.Martin J A and Mak D B. A review of infectious disease screening of refugees by the Migrant
Health Unit, Western Australia in 2003 and 2004;MJA 2006; 185: 607–610.
35. Paxton G A, Sangster K J, Maxwell E L, McBride C R J, Drewe R H. Post-Arrival Health
Screening in Karen Refugees in Australia; PLoS ONE 2012 | 7 | 5 | e38194.
36.http://pdfs.semanticscholar.org. cross-sectional assessment of knowledge, attitude and practice
on hepatitis B and hepatitis C prevalence and risk factors among high risk individuals. Access
at May 16, 2018.
37.Belyhun y, Maier M, Mulu A, Diro E and Liebert U G. Hepatitis viruses in Ethiopia: a
systematic review and meta-analysis: BMC Infectious Diseases 2016 16:761.

39
Annexes

Annex-I. Information sheet


Purpose: To estimate prevalence, KAP and associated risk factors of HBV and HCV infections
among refugees at Pugnido-I refugee camp.

Participation: We are asking you to voluntarily participate in this study. And expected from
everyone is to respond some question and give 5 ml of venous blood. The blood samples are
collected using sterile materials.
Risks: The risks associated with this study could be some discomforts/pain/ when we draw 5ml of
venous blood from you. However, if in case any problems arise during and following sample
collection, we shall offer you necessary medical interventions in this regard.
Benefits: If your status will be positive for HBV and HCV during investigation, result will be
declared to you by investigator to get integrated health education and follow up by contacting the
health institution. If your status will be negative for HBV you can prevent future HBV infection
with dealing to concerned body.
Confidentiality: Information that we will collect from you during this study will be kept
Confidentiality and your identity will be put away after re-coding your file and kept in a secured
place. Only the principal investigators will be able to link your identity with the code number, if
this becomes necessary to assist you in any way.
Sharing the result: At the end of the study we will present the result to responsible bodies, the
report will not bear any information relevant to your personality. We assure you the confidentiality
of such information.
Right to refuse: Since participation in this study is entirely voluntarily, you can refuse to
participate in this study at any time.
Any question regarding this study can be addressed to:
Principal Investigator: Abiyu Ayele
Contact Address: Addis Ababa University, College of Health Sciences, School of Allied Health
Sciences, Department of Medical Laboratory Sciences. Phone (Cell Phone): +251-911 481319.
E-mail:abiyuayele62@gmail.com.

40
Annex - II. Consent Form
I have been requested to participate in a research project that aims to determine the prevalence and
associated risk factors of Hepatitis B and C viruses’ infection in refugees. I have been informed
that all information I will be giving will be kept confidential was provided the Opportunity to ask
questions and given adequate time to rethink the issue. The aim and objectives of the study are
sufficiently clear to me. I have not been pressurized to participate in any way. I understand that
participation in this study is completely voluntary and that I may withdraw from it at any time and
without supplying reasons. I am fully aware that the results of this Study will be used for scientific
purposes and may be published. Agree to this, provided my privacy is guaranteed. And I confirm
my agreement by putting my signature below. I hereby give my consent for giving of blood
specimens.

Full Name: _____________________________________


Signature: ______________________________________
Date: __________________________________________
Address of the investigator
Name: Abiyu Ayele
Address: Addis Ababa University, College of Health Sciences, School of Allied Health Sciences,
Department of Medical Laboratory Sciences.

E-mail: abiyuayele62@gmail.com

41
Annex - III. Questionnaire
For the investigation of the socio-demographic, associated risk factors and KAP of HBV and HCV
infections in refugees at Pugnido-I refugee camps Gambella, Ethiopia.
Participant Code no-------------------
A. Socio-demographic oftheparticipant (circle your answers)
No Question Response Option
1. Sex 1.Female 2.Male
2. Age ………………………
3. Marital status 1. Single 2. Married 3. Divorced, 4. Widowed
4. Education 1. Illiterate 2. Elementary 3. High school,
4. Higher education.
B. Associated risk factors of hepatitis B and C viruses infection
1 Do you have history of multi sexual partner in life? 1. Yes. 2.No.
2 Do you have sharing of sharp materials with others? 1. Yes. 2.No.
3 Do you have history of tattooing? 1. Yes. 2.No.
4 Is there family history of liver disease? 1. Yes. 2.No.
5 Do you have history of tooth extraction? 1. Yes. 2.No.
6 Have you ever taken HBV vaccination? 1.Yes 2.No
C. Participant knowledge towards HBV and HCV infection
No Question Response Option Remark
1 Have you ever heard about HBV and HCV 1.yes 2.No
2 infection?iiiiIinfectionhepatitis/livdisease/?
Is Hepatitis transmitted through sex? 1. Yes. 2. No.
3 Can you get hepatitis infection through body fluid contact? 1. Yes. 2. No.
4 Do HBV and HCV cause liver cancer? 1. Yes. 2. No.
5 Does HBV have vaccine? 1. Yes. 2. No.
6 Is there effective treatment for HBV and HCV? 1.Yes 2.No

D. Participants attitude towards HBV and HCV infection


1 Do you believe HBV &HCV transmitted through food? 1. Yes 2. No
2 Do you think hepatitis infection is curable disease? 1. Yes 2. No
3 Do you believe hepatitis infection is serious public health 1. Yes 2. No
problem
4 Do you think taking HBV vaccine is safe? 1. Yes 2.No

E. Participants practice towards HBV and HCV infection


1 Have you received HBV vaccination?
problemproblem?
2 Have you screened for HBV and HVC?
3 Have you exchange of injection with drug users

Participants name ----------------------------- signature --------------Date------------

42
Annex - IV. Laboratory Results format:
Code --------------------

1. HBs Ag Positive - Negative -

2. Anti-HCV Positive - Negative -

3. ELISA HBV Positive - Negative -

4. ELISA Anti-HCV Positive - Negative -


Remark.________________________________________________________________
____________________________________________________________________________

43
Annex - V. principle and procedure of tests
A) HBsAg rapid test principle:

HBsAg rapid test that utilizes the principle of immunochromathography, unique two site

immunoassay on a membrane. The test sample flows through the membrane assembly of the

cassette, the color monoclonal anti-HBsAg colloidal gold conjugate complexes with HBsAg in the

sample. This complex moves further on the membrane to the test region where it is immobilized

by another monoclonal anti-HBsAg antiserum coated on the membrane leading to formation of a

pink-purple color band which confirms a positive test result. Absence of this color band in the test

region indicates a negative test result. Un reacted conjugate and unbound complex, if any moves

further on the membrane and are subsequently immobilize by the anti-rabbit antibodies coated on

the membrane at the control region, forming a pink/purple color band. This control band serves to

validate the test result [Test kit leaflet].

B) Anti-HCV rapid test principle:

Rapid test is utilizes the principle of immuno-chromathography, unique two site immunoassay on

a membrane. As the sample flow through the membrane of the test strip, the test color HCV antigen

colloidal gold conjugate complexes with anti-HCV in the sample. This complex moves further on

the membrane to the test region where it is immobilized by another HCV antigen coated on the

membrane leading to formation of a pink-purple color band which confirms a positive test result.

Absence of this color band in the test region indicates a negative test result. Un react conjugate

and unbound complexes, if any moves further on the membrane and are subsequently immobilize

by the anti-HCV coated on the membrane at the control region, forming a pink/purple color band.

This control band serves to validate the test result [Test kit leaflet].

C) Procedures for HBV and HCV rapid tests


44
1. Before sample collection introduce yourself and identify the patient
2. Take a time to wash your hands and wear gloves
3. Prepare the material required (needles, tubes, etc.)
4. Prepare the patient
5. Apply the tourniquet (do not let it on for extended period)
6. Choose a vein
7. Disinfect the draw site
8. Collect serum specimen in a clean test tubes.
 Ensure that only sufficient quantity of the specimen is collected.
 Exit the vein and apply pressure
 Discard the needle(in appropriate biohazard container)
 Label the specimen before leaving the patient
 Check the patient apply a plaster if necessary
 Allow the specimen for 30 minutes to facilitate clotting-
 Centrifuge with medium speed for 10 minutes
 Separate serum from the blood by Pasture pipette
 Perform the lab test and store the remaining serum at -200c
9. Bring the sealed pouch to room temperature, open the pouch and remove the cassette/strip
Once opened, the cassette must be used immediately.
10. Measure 50 micron serum with pipette and dispense the sample in sample well.
11. The cassette/strip should be left to horizon until the specimen flow evenly distributed.
12. At the end of the given time based on the manufacturer instruction read the result as follows:
 NEGATIVE: Only one colored band appears on the cassette
 POSITIVE: two distinct colored bands appear on the cassette.
13. The test should be considered invalid if no band appears. Repeat the test with a new
cassette/strip.
14. Although, depending on the concentration of HBsAg in the specimen, positive results
may be start appearing as early as 2min, negative results must be confirmed only at the end
of given time.
15. In case of a doubtful result at final time, the test may be extended up to 30min to get a clear
back ground.

45
D)HBsAg ELISA test principle

This is a Sandwich Enzyme linked Immunosorbent assay method in which polystyrene microwell
strips are pre-coated with monoclonal antibodies specific to HBsAg. Donor’s serum or plasma
sample is added to the microwells together with a secondary antibody conjugated with horseradish
peroxidase (HRP) and directed against a different epitope of HBsAg. During incubation, the
specific immune-complex formed in the case of presence of HBsAg in the sample, is captured on
the solid phase. After washing to remove sample serum protein and unbound HPR-conjugate,
chromogen solution containing tetramethylbenzidine (TMB) and urea peroxidase are added to the
walls. In the presence of the antibody-antigen-antibody (HRP) sandwich immune-complex, the
colorless chromogens are hydrolyzed by the bound HPR conjugate a blue colored product. The
blue color turns to yellow after stopping the reaction with sulfuric acid. The amount of color can
be measured and is proportional to the amount of antigen in the sample (Test kit leaflet).

E) Anti-HCV ELISA test principle


Polystyrene microwell stripes are pre-coated with recombinant, highly immune-reactive antigens
corresponding to the core and non-structural regions of HCV. During the first incubation step, anti-
HCV specific antibodies, if present, will be bound to the phase pre coated HCV antigens. The
wells are washed to remove unbound serum proteins, and rabbit antihuman IgG antibodies (anti-
IgG) conjugated to HRP is added. During the second incubation step, these HRP conjugated
antibodies will be bound to any antigen- antibodies complexes previously formed and the unbound
HRP-conjugate is then removed by washing. Chromogen solutions containing TMB and urea
peroxidase are added to the wells and in presence of the antigen-antibody-anti-IgG (HRP) immune-
complex; the colorless chromogens are hydrolyzed by the bound HRP-conjugated to a blue colored
product. The blue color turns to yellow after stopping the reaction with sulfuric acid. The amount
of color can be measured and is proportional to the amount of antibody in the sample (Test kit
leaflet).

46
F) Test Procedures for ELISA

1. A micro titration well plate is coated with known antigen.

2. Add patent’s serum. If the serum contains antibody it combine with antigen.

3. Wash carefully by using automatic washer more than 6 times.

4. Add enzyme labeled antihuman globulin, which attaches to the antibody.

5. Wash carefully.

6. Add the substrate, which is hydrolyzed (broken down) by the enzyme to give a color change.

7. Read the result.

47
Annex .VI. Thesis declaration
I the undersigned agree to accept all responsibilities for the scientific and ethical conduct of the
research project. I was provided timely progress report to my advisor and seek the necessary advice
and approval from my primary advisors in the course of the research. I was communicated timely
to my advisors and all stakeholders involved in the study.
Name of the principal investigator:
Abiyu Ayele (BSc) Signature____________________ Date _________________
Name of Advisors:
1.Mr- Kasu Desta( Bsc, Msc, PhD fellow, Associate professor)
Signature __________________Date___________________
2.Mr. Melese Hailu (Bsc ,MSc, PhD fellow)
Signature _____________________Date_____________________

48

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