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Attachment 4: Protocol for
Prevalence,
Incidence, Epidemiology and Molecular Variants of HIV in Blood Donors
in Brazil
OMB Number: 0925-0597
Abstract
Establishing
and monitoring viral prevalence and incidence rates, and identifying
behavioral risk behaviors for HIV incidence among donors, are
critical steps to assessing and reducing risk of HIV transmission
through blood transfusion. Identifying donation samples from donors
with recent HIV infection is particularly critical as it enables
characterization of the viral subtypes currently transmitted within
the screened population and hence most likely to "break-through"
routine screening measures (i.e., peri-seroconversion window period
donations). In addition to characterizing genotypes of recently
infected donors for purposes of blood safety, molecular surveillance
of incident HIV infections in blood donors enables documentation of
the rates of primary transmission of anti-viral drug resistant
strains in the community, and serves a public health role in
identifying new HIV infections for anti-retroviral treatment. We
plan to enroll
eligible HIV positive subjects detected at our four blood centers:
Sao Paulo, Recife, Rio de Janeiro and Belo Horizonte, and analyze
molecular variants and their correlation with risk behaviors. Aims.
Determine risk factors associated with HIV infection, HIV subtype,
and drug resistance profile among HIV positive donors according to
HIV infection status (nucleic acid testing (NAT) yield versus recent
versus long-standing
seropositives), year of donation and site of collection.
Previously we conducted a case
control study of HIV seropositive donors and a comparison population
of uninfected donors as part of the NHLBI-funded Retrovirus
Epidemiology Donor Study (REDS-II) International Brazil. The new
study will build off of the previous study to continue risk behavior
and molecular surveillance at the four REDS-III blood centers. Note
that the formal name of the study has changed to Recipient
Epidemiology and Donor Evaluation Study (REDS-III), but our study
objectives for this HIV project remain similar to the previous
REDS-II study.
NAT testing for HIV (and HCV)
is currently being implemented in Brazil. It will be important to
continue to collect molecular surveillance and risk factor data on
HIV infections, especially now that infections that might have been
missed by serology testing will be identified through the use of NAT.
NAT-only infections represent recently acquired infections. Therefore
the results of our HIV surveillance study will be especially useful
for interpreting the findings of HIV NAT testing in Brazil. For
example, HIV test seeking at blood banks is already a concern. If we
find that NAT-only donors are test seeking this will raise critical
policy issues. Even after NAT is implemented, the residual risk of
HIV infection is likely to remain substantially higher than in the
USA because of the approximately 10-fold prevalence of infection in
Brazil compared to the USA. Additional measures towards safe donor
recruitment and deferral continue to be essential in further reducing
the risk of transfusion-transmitted HIV infection. The continuation
of these important HIV activities will build directly off of the
capacity established at all 4 blood centers during participation in
the REDS-II Brazil HIV case control study.
Specific
Aims
Aim. Determine risk factors
associated with HIV infection, HIV subtype, and drug resistance
profile among HIV positive donors according to HIV infection status
(NAT yield vs recent vs
long-standing
seropositives), year of donation and site of collection.
Hypothesis 1: Having
multiple heterosexual partners, male-to-male sex, and toa lesser
extent injection drug use (IDU) will continue to be the predominant
risk factors for HIV in Brazil among both seroprevalent infections
and incident infections detected by NAT or recent seroconversion.
Hypothesis 2: There will be
clinically relevant increases in the diversity of HIV subtypes and
increasing rates of primary drug resistance among recently infected
donors in all 4 blood centers. Non-B subtypes and drug resistant
strains will be seen in recently infected persons from all risk
factor categories.
Background
The HIV epidemic continues to
be a major public health problem in Brazil. The HIV/AIDS epidemic
began in Brazil in the early 1980s, and Brazil now has the largest
HIV-1 infected population in South America, with 544,846 reported
cases of AIDS and 630,000 individuals known to be living with HIV in
2009��1�.
The
epidemic in Brazil is considered a
“concentrated epidemic”, with an overall prevalence below
1% in the general population��2�,
but levels as high as 50% among vulnerable population such as males
who have sex with males (MSM), injection drug users (IDUs) or sex
workers ��3�.
Incidence of AIDS cases vary across Brazilian regions, with the
highest incidence rates concentrated in the South and the Southeast
(29.3 and
19.2/100,000),
followed by the Midwest, North and Northwest (16.4;
15.4; and 11/100,000��1�.
Although
incidence of AIDS has stabilized in the South, Southeast and Midwest,
HIV transmission and clinical AIDS case report rates are increasing
in the North and Northeast. According to the criteria of the World
Health Organization (WHO), Brazil has an HIV epidemic with prevalence
of HIV infection of 0.6% in 15 to 49 year old age strata, and
concentrated foci in specific sub-populations with prevalence greater
than 5%. In 2005, 35,965 new cases of AIDS were reported,
representing an incidence rate of 19.5 AIDS cases per 100,000
inhabitants. Sao Paulo, Rio de Janeiro and Minas Gerais States (all
in the Southeast) are responsible for 64% of AIDS cases in Brazil,
while Pernambuco (in the Northeast) has a higher rate of new
infections than the other regions��1�.
Studies evaluating the prevalence of drug-resistant virus among
recently infected individuals are thus extremely important in Brazil.
A survey developed by the Brazilian Ministry of Health which included
535 patients from the entire country, found that the frequency of
primary resistance was low, 4.4% for nucleoside reverse transcriptase
inhibitors (NRTI) and non-nucleoside reverse transcriptase inhibitors
(NNRTI) and 2.2% for protease inhibitors��4�.
(Dr Sabino was a co-investigator on this project.) More recently,
Sucupira and colleagues analyzed 75 drug naïve HIV positive
individuals in the city of Santos and found 21 (28%) harboring
resistant strains, raising grave concern that in certain areas of
Brazil drug resistant strains may be rapidly increasing and
spreading��5�.
HIV/AIDS
health care in Brazil is provided by the state to all HIV infected
individuals. As early as 1991, the Brazilian Ministry of Health
provided antiretroviral (ARV) drugs through its extensive public
health system. In 1996 a law was enacted guaranteeing free access of
antiretroviral therapy to all Brazilians who required treatment,
according to Brazilian guidelines. The widespread use of ARV has led
to a decline in AIDS related mortality in Brazil��6,7�.
However, it is expected that the proportion of patients experiencing
virologic failure and consequently harboring resistant strains will
increase in time. Depending on the behavioral characteristic of these
individuals, transmission of drug resistant strains may occur with
increased frequency��8�.
The transmission of resistant variants to uninfected individuals
raises serious clinical and public health consequences and may
dramatically impair the capacity of treating HIV in the near
future��9-14�.
Moreover, the
genetics of the virus can be used to track the movement of HIV-1 into
new groups or new at-risk populations. It is also conceivable that
the diversity of the virus may impair the immune response to
candidate vaccines, cause false negative results in blood screening,
diagnostic and monitoring laboratory tests (e.g. especially viral
load assays targeting nucleic acids)��15,16�,and
lead to differences in the observed disease progression��11�,��10�
and therapeutic response��14,17�.
The predominant HIV-1 clade in Brazil is B (~70%), but unlike the
U.S., Brazil also has appreciable numbers of HIV-1 infections caused
by clade F (~15%), C (~3%), and circulating recombinant forms (CRFs,
~12%).��18-20�
Furthermore, approximately 50% of the clade B strains circulating in
Brazil comprise a cluster of genetically and antigenically distinct
strains relative to US clade B strains��21�.
Monitoring HIV viral subtypes and drug resistance patterns, and
identifying risk behaviors for incident HIV infections among donors
(NAT yield and recent seroconvertors) are critical steps to assessing
and reducing risk of HIV transmission through transfusion��22�.
In addition to characterizing genotypes of recently infected donors
for purposes of blood safety, molecular surveillance of HIV
infections in blood donors enables documentation of the rates of
primary transmission of anti-viral drug resistant strains in the
community, and serves a public health role in identifying new HIV
infections for which subjects can then obtain anti-retroviral
treatment.
In Brazil��23�
the prevalence and incidence of HIV infection varies widely by
geographic area and by demographic and behavioral subgroup. In this
sense, it is essential at the State and local levels that HIV
prevention activities be targeted to those geographic areas and
population groups currently affected by HIV and to those into which
the virus may be spreading. The impact of prevention activities is
reflected in the prevalence and trends of infection over time. At
regional and national levels, knowledge of the current patterns of
HIV infection and estimates of the total number of infected persons
are important for anticipating future health needs and setting
public health policies in
Brazil.
Enrollment
in the REDS-II HIV study is closed and we are currently analyzing the
data. A total of 343 HIV positive blood donors and 901 HIV
seronegative controls enrolled in the study. Data reporting molecular
variants and demographic characteristics of HIV positive donors was
presented at the 2011 AABB meeting held in San Diego. Of clear
concern, thirty-two of 343 cases were taking anti-retroviral therapy.
These donors were excluded from the analysis of primary transmitted
drug resistance. A total of 274 samples could be typed and the
distribution by subtype is shown the table below. Non-B subtypes
represent a quarter of HIV infections in the blood donor at the four
REDS-II blood centers. Thirty-six of the 274 subtypes (13%) had
evidence of primary drug resistance. Specific demographic and
behavior risk factors were not associated with primary drug
resistance. Further analyses are underway at this time.
Total number of specimens
available for subtyping
|
Subtypes
n (%)
|
A
|
B
|
C
|
F
|
C/F
|
B/F
|
274
|
1 (0.4)
|
212 (77)
|
13 (5)
|
37 (14)
|
2 (1)
|
9 (4)
|
With
respect to the larger HIV risk factor analysis, preliminary results
suggest that the use of audio computer assisted self-interview
(ACASI) methodology has been very important for disclosure of risks
because even seronegative donors disclosed deferrable risk behaviors.
This by itself has important implications for blood safety in Brazil.
Significance
Defining
prevalence and incidence in blood donors and residual risk of HIV
transmission by transfusions in Brazil may lead to new blood safety
approaches in Brazil. The data we will collect can be used to project
the yield, safety impact and cost-effectiveness of implementing
enhanced testing strategies that include nucleic acid testing..
Determination of HIV risk factors in donors according to additional
characteristics (first time versus repeat donor status; volunteer
versus replacement status; demographics and risk behaviors) will
support policy discussions over strategies to recruit the safest
possible donors in Brazil, and will also yield significant
information for HIV surveillance in Brazil when combined with
prevalence and incidence data derived from general populations and
high risk surveillance studies. The documentation of incident HIV
infections allows for clinical identification of recently transmitted
strains of virus in donor settings in the different cities of Brazil.
This surveillance will monitor the trafficking of non-B subtypes and
rates of transmission of drug resistant viral strains in low risk
blood donors that can be compared with data from similar studies in
higher risk populations. Monitoring drug resistance strains is
extremely important in a country that provides free ARV therapy for
HIV infected individuals, many of whom have low level education and
modest resources, thus making compliance with drug regimens and hence
the risk of drug resistant HIV a serious problem. The findings from
this project will also complement similar monitoring of HIV
prevalence, incidence, transfusion risk and molecular variants in the
USA and other funded international REDS-III sites in South Africa and
China, thus allowing direct comparisons of these parameters on a
global level.
By combining HIV data collected in Brazil during REDS-II and REDS-III
we will also be able to
examine time trends in HIV molecular variants and risk factors
associated with HIV infection in donors from 2007 through to 2017.
Approach
All
blood donations are routinely screened by two HIV-1 antibody assays
in parallel, as mandated in Brazil. These assays have been selected
to have comparably high sensitivity to early seroconversion and
diverse clades, as well as excellent specificity with non-overlapping
populations of false reactivity. Samples reactive by both EIAs will
be considered positive for prevalence calculations. In Brazil, only
subjects who return for counseling will have a follow-up sample
obtained that will be tested by western blot (WB) (~80% of HIV
reactive subjects return and WB is performed, of which 95% confirm as
WB positive). In addition, a NAT screening assay for HIV and HCV in
pools of 6 donations has been developed for use in blood centers in
Brazil. The NAT assay will be used at all of the REDS-III blood
centers in Brazil during the planned HIV case surveillance
activities. In addition, to
detect recently infected donations, samples from all HIV dual-EIA
reactive donations and/or NAT positive donations will be tested by
the Recent Infection Testing Algorithm (RITA)
which is based on use of a sensitive/less-sensitive enzyme
immunoassay ("detuned" EIA)��24,25�.
RITA
testing
will be performed by BSRI
(Blood Systems Research Institute, the REDS-III Central Laboratory)
because these test kits are not registered for use in Brazil and
would be difficult for the local laboratory to import. For enrolled
subjects, this testing will be performed on linked index and
enrollment specimens from WB-confirmed donors, whereas for subjects
who do not return for counseling we will anonymize the donation
samples. False positive samples will be identified by performing
sensitive EIA and WB on samples lacking reactivity on the LS-EIA
(i.e., standardized optical density <0.1). Incidence data derived
using the RITA methods will be used to project risk and yield of
enhanced donor screening strategies. Subtype and drug resistance
profiles will be determined in Dr. Sabino’s laboratory on all
donors who returned for counseling and consented and enrolled into
the interview study (see below). Risk factors and donor demographics
will be correlated with recent infection status, as well as with
clade and acquisition of drug resistant virus.
This
study will be conducted at all four participating REDS III centers
in Brazil; Sao Paulo, Recife, Rio de Janeiro and Belo Horizonte.
Methods
Study
Design.
Surveillance of all HIV positives during a period of 5 years,
with serological confirmation and RITA, will allow calculation of HIV
prevalence and incidence. A detailed risk factor questionnaire
testing for HIV genotype, and drug resistance will be done on all
consented HIV cases. Data analysis will compare the frequency of
reported risk behaviors between first-time vs
repeat donors, community vs
replacement,
recent vs long standing infections, year
of donation and site of collection.
Secondary
analyses will provide evidence
for changes (declining or increasing) HIV prevalence and incidence in
selected sites and explore the reasons for the changing patterns in
particular the role of behavioral change; and also evaluate if the
frequency of specific risk factors in the blood donor population such
as MSM, multiple heterosexual partners, and IVDU are changing over
time. [To assess this, we will compare REDS-II HIV case risk factors
to those we determine using the identical ACASI in REDS-III]Analyses
on the cumulative data will be repeated at annual intervals to assess
secular trends in HIV risk factors.
Study
Population.
Surveillance
will be performed to identify HIV NAT yield cases and HIV
seropositive donors. All eligible cases will previously have had dual
HIV EIA testing, NAT and Western blot performed to confirm their HIV
seropositivity, per core REDS-III procedures at Fundação
Pró Sangue/Hemocentro de São Paulo. Recently infected
individuals will be defined through the Standardized Testing
Algorithm for Recent HIV Seroconversion (RITA) protocol. An ACASI on
risk factors, developed for REDS-II and in place at all 4 centers,
will be administered to subjects who return for counseling and
consent to participate in the study. Testing for HIV genotypes and
drug resistance will be performed on all consented HIV cases at
Fundação Pró Sangue/Hemocentro de São
Paulo as previously described. The genotype result will be sent to
the donor by mail and they will be counseled to take it to their
physician. If desired by the subject a new visit will be provided to
discuss the results of genotype testing. We plan to enroll 25 cases
per year at each center or approximately 1 case every other week. For
these subjects, in addition to Western blot testing, we will perform
linked genotype and drug resistance testing on the sample obtained at
the time of counseling. For those individuals who do not return for
confirmatory testing, the samples will be anonymized and tested using
RITA.
Inclusion
& Exclusion Criteria.
Portuguese-speaking
blood donors aged 18–65 years at the four participating blood
centers who were confirmed HIV-positive by EIA or NAT and Western
blot. Autologous blood donors will be excluded.
Subject
Enrollment:
Subjects will be enrolled for a 5-year period from March (or when
OMB approval is received) 2012 – 2017. According to the
Brazilian guidelines blood donors are requested to return to the
blood bank for confirmatory testing (Western blot) and HIV
counseling. At the time the donors return for the final HIV results
and counseling and they will be invited to participate in the study,
and if consent is obtained the ACASI questionnaire about risk factors
and motivations to donate will be administered. For these subjects,
we will perform linked genotype and drug resistance testing on the
sample obtained at the time of counseling. For those individuals
that do not return for confirmatory testing, the samples will be
anonymized and sent to BSRI to perform the RITA.
Procedures:
A
-Questionnaire
A
detailed HIV risk factor questionnaire will be administered to all
subjects. This is the same instrument that was previously used in
REDS-II except for a change in the name of the instrument and removal
of one of the data capture fields that was used by study research
assistants to define case or control status for the REDS-II study. As
the REDS-III case surveillance study will only include HIV positive
donors this data capture field is no longer necessary. A
self-administered audio computer-assisted self-interview (ACASI) on a
laptop computer will continued to be used in order to maximize
reporting of stigmatized or socially sensitive behaviors. A research
assistant or nurse will provide the ACASI laptop (including earphones
to be able to listen to the questions confidentially) to each subject
at the blood center. The study subject will be shown how to use the
computer to complete the interview by entering
basic demographic data with the help of the research assistant or
nurse,
but will be given privacy to complete the rest of the questionnaire.
The research assistant or nurse will remain available to answer
questions and provide help as necessary.
B
- Phlebotomy for Clinical Testing
In addition to blood saved
from their index blood donation, 30 ml of blood will be drawn from
cases at the time of the enrollment and interview. Specimens
will be sent to Sao Paulo for genotype testing and to the USA for
RITA testing, and the remaining specimens will be processed into
aliquots and saved in the study repository in Sao Paulo for future
testing, including repeated genotyping and drug resistance, if
necessary. Specimens will be stored in Brazil in accord with
Brazilian law. Specimens sent to the USA for RITA will be kept until
the study is concluded (March 20, 2018). On this date remaining
specimens and residual aliquot volumes in the USA will be destroyed.
C
- Detection of Recent Infections by Less Sensitive-Enzyme Immunoassay
(LS-EIA) Testing
All
eligible cases will previously have had dual HIV EIA testing and HIV
Western blot to confirm their HIV seropositivity, per core procedures
at our Brazilian central lab. Recently infected individuals will be
defined through RITA testing at BSRI in San Francisco, CA, USA.
D
- HIV-1 Clade Typing and Drug Resistance Testing
Subtype
and resistance analysis will be performed at Fundação
Pró Sangue Hemocentro de São Paulo as previously
described��25,26�.
Sequencing of the entire HIV-1 protease gene (99 amino acids [aa])
and of the RT gene through amino acid 240 will identify all mutations
known to confer resistance to protease, nucleoside and non-nucleoside
RT inhibitors ��26�.
The only class of approved anti-HIV-1 drug resistance not detected by
this analysis will be envelope gene mutations known to confer
resistance to the more recently introduced HIV-1 fusion inhibitor
FuzeonTM,
a drug that is not yet in use in Brazil. Following phylogenetic
analysis, sequencing of the pro-RT region will also identify the
subtype of the recently transmitted HIV-1 strain. RNA
will be isolated using QIAamp Viral RNA Mini kit (Qiagen Inc.,
Valencia, CA) according to the manufacturer's instructions.
Complementary DNA will be obtained using Superscript reverse
transcriptase (Invitrogen, Carlsbad, CA) and random primers
(Pharmacia, Uppsala, Sweden). A nested PCR will be used to obtain one
fragment containing the protease gene and approximately 700 base
pairs of the RT gene. In the first round the primers K1/K2 will be
used followed by DP10 and F2 primers.31
Three other sets of primers, RT4/DP16, F1/F2 and DP10/DP11, will be
used for samples that are not amplified using the initial primers.
Conditions for both rounds of PCR will be 94°C for 1 minute
followed by 35 cycles at 94°C for 45 seconds, 55°C for 45
seconds and 72°C for 2 minutes, with a final elongation step at
72°C for 10 minutes All amplification products will be analyzed
on a 1% ethidium bromide-stained agarose gel. PCR products will be
purified using QIAquick PCR purification kit (Qiagen Inc.). To obtain
sequence results for the entire amplified segment in both strands we
will use at least 6 primers for sequencing each sample, including F1,
F2, DP10 and DP11 primers and a new pair of primers - GABO 1 (sense
-5' -CTC ARG ACT TYT GGG AAG TTC- 3') and GABO-2 (antisense - 5' -GCA
TCH CCC ACA TCY AGT ACT G-3' ). Sequence data will be obtained using
the ABI Prism Big Dye Terminator Cycle Sequencing Ready Reaction kit
(Applied BioSystems Inc., Foster City, CA, USA), according to
manufacturer's protocol in an automated sequencer (ABI 377
Sequencer-Applied Biosystems). To detect possible PCR contamination,
sequences will be compared to each other using a web interface that
uses the Blast program and which highlights any pair of sequences
that have a percentage of similarity higher that a specific threshold
(we will use 99% for pol gene)��15,16�.
Counseling
and Medical Referral.
Prior to
enrollment, all subjects will have received counseling regarding
their HIV infection by trained personnel at the blood centers, per
operational protocols. The genotype result will be sent to the donor
by mail and they will be counseled to take it to their physician. If
desired
by the subject a
new visit will be provided to discuss the results of genotype
testing.
Data
Analysis
Analysis
of Incidence, Residual Risk and NAT Yield.
Data
analysis will be performed by the REDS-III data coordinating center,
Research
Triangle Institute-RTI
International in Rockville, Maryland, US. Data from this study will
be merged with the large Brazilian donation database to allow
calculation of incidence and univariate and multivariate analysis of
correlates of HIV incidence and calculation of residual risk and
yield of NAT. Since Clade B is responsible for more than 80% of the
infections in Brazil, we will assume the window period corresponding
to the time from seroconversion by sensitive EIA and Western blot to
seroconversion by the LS-EIA would be similar to that reported for
U.S. clade B infected persons, i.e., 170 days (95% confidence
interval [CI] 145-200 days). We will further assume that the
detection window periods (period from infectivity by blood
transfusion to initial detection by the respective markers) for viral
RNA by ID-NAT, MP-NAT, p24 antigen and antibody EIAs were 5.6, 9.0,
15.0 and 20.3 days, respectively, as described by Busch et al��24�.
Based on our observed incidence rates and the published WP estimates,
the predicted yield and associated residual risk (per 10,000 per
year) for each test will be calculated using the formula: (incidence
rate) ∕ (365)
(detection window period). The statistical calculations will use the
method of Busch, et al as follows. Confidence intervals for
prevalence rates will assume prevalent cases are binomially
distributed. Logistic regression will be used to assess differences
in prevalence rates by year, type of donation, gender, and age.
Confidence intervals for incidence rates will assume incident cases
are Poisson distributed.
The
findings from this project will add to those obtained in the REDS-II
study, allowing for extended trend analyses over a 10-year period and
will complement similar monitoring of HIV prevalence, incidence,
transfusion risk and molecular variants in Brazil. Poisson regression
will be used to assess differences in prevalence rates by year, type
of donation, gender, and age. Wald type 95% confidence intervals
around residual risk estimates and yield estimates will be computed
using a Taylor series approximation to the residual risk standard
error estimates and yield standard error estimates. These standard
errors are a function of the standard errors of the Poisson
distributed incidence rates and the standard error of the window
periods.
Analysis
of Risk Behaviors.
Independent
variables will be HIV risk factors ascertained by questionnaire,
including male-to-male sex, number of lifetime male and female sexual
partners, number of male and female sexual partners within the past
year, use of condoms, sex with a prostitute or sex work by the donor
him/herself, IDU, sex with an IDU, and sex with an individual known
to be HIV-positive. Secondary predictors will include demographics,
socioeconomic status, drug and alcohol use. Subgroup analyses will
be done in males and females and in volunteer and replacement donors,
first-time and repeat donors. Data from the questionnaire will also
be used in analyses of HIV subtypes and drug resistance, below. We
will report the frequency of risk behaviors according to demographic
characteristics, recent versus long-standing infection, and HIV
genotype categories. Univariate associations of specific risk factors
and recent infection compared to longstanding infection will be
assessed using contingency tables with significance tests using Chi
squared or Fisher's exact tests. Variables with significant or
borderline univariate associations (p<0.10) with HIV
seropositivity will be entered into a logistic regression model to
assess independent associations and potential confounding.
HIV
Subtype and Drug Resistance Analyses.
To
define the subtype of each strain we will use interface software that
automatically submits the sequences to two programs: RIP��27�
and Blast��28�.In
the RIP program, the sequence is cut in fragments of 200 bp in 1 bp
steps. Each fragment is compared to a set of reference strains and
for each fragment the program determines which reference sequence has
the highest similarity rate to that fragment. In the Blast approach,
the sequence is cut into non-overlapping fragments of 200 bp. Each
fragment is submitted to a bank of 10,000 sequences previously
subtyped in the Los Alamos databank. The program detects which
databank sequence is most similar to each fragment. If the results of
both analysis agreed, the sample will be considered subtyped.
Otherwise the sequence will be manually reviewed using SIMPLOT��29�.
Interpretation
of results identifying possible Protease and RT mutations that have
been associated with reduced antiretroviral-drug susceptibility will
be based on the International AIDS Society classification��30�
Protease: D30N; M46I; M46L; G48V; I50V; V82A; V82S; V82F; V82T; I84V
and I90M. Reverse Transcriptase: M41L; A62V; K65R; D67N; T69D; 69
insert; K70R; L74V; V75I; V75T; V75M; V75S; V75A; F77L; A98G, L100I;
K103N; V106A; V108I; Y115F; F116Y; Q151M; Y181C; Y181I; M184V; M184I;
Y188C; Y188L; Y188H; Y188C; G190A; G190S; L210W; T215Y; T215F; K219Q;
K219E; P255H; P230L and P236L. Reverse transcriptase mutations that
are different from wild-type T215 and T69A/N/S will be included as
well.
Sample
Size and REDS-III Enrollment:
Our experience in REDS-II was
the following:
Overall Enrollment in the
REDS-II International Component Brazil HIV Case Control Study.
Subject Type
|
Identified
|
No Response to recruitment
Letter
|
Refused
|
Withdrew or Dropped out
|
Final Enrollment
|
Case
|
564
|
181
|
27
|
13
|
343
|
Control
|
N/A*
|
352
|
18
|
24
|
901
|
*The identified control
population is total of number of accepted blood donors who
successfully donated and screened negative for all infectious
markers.
Of all
potential HIV positive subjects during the REDS-II study period at
the four blood centers we were able to enroll 60%. Of those who
responded to our recruitment efforts, nearly 90% are included I our
final enrollment numbers.
Based on REDS-II experience,
we expect that as many as 10 NAT-only yield cases and 200 HIV
Ab-positive donors per year will be identified through standard
testing at the 4 blood centers in REDS-III. All 200 seropositive
donors will be tested for recent acquisition of infection (rapid
detuned testing). We are assuming that 50% of these donors
(approximately 100) will participate in this study, completing the
ACASI risk factor interview and additional sample collection for
viral subtype and resistance testing. Over the proposed enrollment
period of 5 years this
will provide risk factor and surveillance data for 500 HIV-positive
donors.
Expected
Results.
Based upon our preliminary data, we expect to find that male-to-male
sex and multiple heterosexual partners remain risk factors for HIV.
With the larger sample size, we shall have better power to analyze
risk factor profiles separately in volunteer vs. replacement blood
donors. Given their age and socioeconomic status, we hypothesize that
under-reported IVDU in the heterosexual population explain the
unexpectedly high HIV prevalence in volunteer donors.
Potential
Nonresponse Bias
During
data collection, we will monitor participation and response rates to
identify any potential problems that are indicated by differential
response rates across sites. We assume that the responses rates HIV
positive subjects for the completed REDS-II and planned REDS-III
phases of the study will be similar. We will conduct nonresponse bias
analysis to assess the potential for nonresponse bias. If we find
that nonresponse bias may exist, we will conduct post-survey
weighting based on the information produced during the nonresponse
bias analysis to minimize the potential nonresponse bias when the
risk behavior frequencies are reported. The factors that could
be associated with non-participation and nonresponse are demographic
characteristics of the donors (age, gender, race/ethnicity, previous
donation history) and also potential participation rate differences
by blood center. It is important to note that simple or unadjusted
HIV case rates per site will not be sufficient to indicate whether
there is evidence of bias because the demographic characteristics of
blood donors at each of the REDS-III blood centers are not the same.
We
expect low levels of item nonresponse for this study. Our use of
ACASI was very successful in the previous REDS-II study with little
evidence of important levels of nonresponse to any of the questions
asked during the interview. For example, we asked a question about
whether the donor had ever been tested for HIV outside of blood
donation. Only 1 person out of 1244 respondents (<0.1%) refused to
answer this question. Similarly, for a clearly social sensitive
question in which we asked respondents to classify their sexual
orientation 18 out 1244 respondents (1.4%) refused to answer. These
data suggest that the use of ACASI was successful in eliciting
responses to stigmatizing or socially sensitive questions, and we
expect the same to be true for our use of the same interview in the
REDS-III HIV case surveillance study.
Human
Subjects Considerations.
This
project will be approved by the institutional review boards (ethics
committees) in Brazil and the U.S. before implementation. The
main risks of this study are: 1) possible lost confidentiality
regarding HIV status or risk behaviors; 2) possible discomfort due to
the personal nature of the questionnaire; and 3) possible negative
information risk of drug genotype test. Benefits of the study
include: 1) HIV positives will receive additional HIV counseling as
part of the study; 2) their clinical treatment may be improved by
providing drug genotype test; and 3) benefits to Brazilian society as
a whole by virtue of potential improvement blood safety and control
of the HIV epidemic and 4) Provide at
regional and national levels, knowledge of the current patterns of
HIV infection and estimates of the total number of infected persons
are important for anticipating future health needs and setting public
health policies.
We shall
attempt to minimize risks by stringent privacy protection of the
subjects’ data (see elsewhere in this application). All data
will be kept on secure, password protected computers and no personal
identifying information will be kept on computers used for this
study. Secure data transfers procedures will be used at all stages
when data is transferred from one computer or participating
organization to another. For example, secure, password protected FTP
procedures will be used when we transfer risk factor and HIV subtype
and drug resistance information to the US DCC. We will also seek to
mitigate discomfort by providing counseling and medical referral for
HIV infection. Informed written consent will be obtained from all
subjects prior to enrollment.
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| File Type | application/msword |
| File Title | HIV positive donors |
| Author | BSRI Employee |
| Last Modified By | Flicker, Laura |
| File Modified | 2014-10-03 |
| File Created | 2014-09-29 |