A Phase II, Randomized, Safety and Immunogenicity Study of a Re-Derived, Live-Attenuated Dengue Virus Vaccine in Healthy Adults

Study design.

This study was a phase II, randomized, single-center, observer-blind, controlled, parallel-group trial conducted in the United States. The study was designed to evaluate the safety and immunogenicity of two formulations of a new live-attenuated tetravalent DENV vaccine compared with a precursor live-attenuated tetravalent DENV vaccine and a cell culture medium placebo.

The study was conducted in two stages. The first stage was an observer-blind evaluation of the above four treatment groups followed for 6 months after administration of a first vaccine dose and 3 months after administration of a second vaccine dose. Subjects were randomly allocated to treatment groups using a 1:1:1:1 ratio. The randomization was performed at GlaxoSmithKline Vaccines, Rixensart, Belgium, using a standard Statistical Analysis System (SAS) program (SAS Institute Inc., Cary, NC).

During this first stage, although the vaccine preparer/administrator was aware of some treatment assignments because of a unique method for preparation of the precursor vaccine (monovalent vials mixed into a tetravalent mixture), no volunteer or investigator was aware of treatment assignments until data collection was completed and the first-stage database was frozen for analysis.

The second stage was an open-label evaluation of a subset of subjects in the two new vaccine treatment groups who consented to receive a third dose of the same formulation used for their primary immunization. The third dose was given 5–12 months after the second dose.

The institutional review board, US Army Human Subjects Research Review Board, Office of the Surgeon General approved the study protocol and supporting documents. The study was conducted between April of 2006 and March of 2008 in accordance with the provisions of the Declaration of Helsinki, Good Clinical Practices, and US regulations. The US Army Medical Materiel Development Activity (USAMMDA) and GSK monitored the conduct of the trial and verified the data. Internal audits by separate teams from the US Army and GSK were also conducted. Written informed consent was obtained from each volunteer before the performance of any study procedures.

Role of the sponsor and development partners.

The study was designed by the US Army and GSK. The USAMMDA, as the sponsor's representative, monitored and reported on subject safety. Investigators collected and encoded the data into a GSK database, and a GSK statistician analyzed the data according to a pre-specified and mutually approved plan. All authors had complete and unfettered access to the data, reviewed the manuscript, and can vouch for the document's accuracy and completeness. The study was jointly funded by the US Army Medical Research and Materiel Command and GSK.

Vaccines.

In this trial, two different formulations of a new live-attenuated tetravalent DENV vaccine designated TDEN (formulations F17 and F19) were compared with the legacy live-attenuated tetravalent DENV vaccine candidate designated F17/Pre10,11 and a cell culture medium placebo. The TDEN vaccine was made using virus seeds re-derived from the F17/Pre vaccine: DENV-1 (West Pac 74, 45AZ5, PDK-27), DENV-2 (S16803, PDK-50), DENV-3 (CH53489, PDK-20), and DENV-4 (341750, PDK-6). Briefly, purified viral RNA from each F17/Pre vaccine virus strain was extracted and used to transfect FRhL cells, the production cell substrate for the F17/Pre vaccine. Progeny viruses from the transfection were then used to produce master and working seeds and finally, new monovalent vaccine lots; these lots were formulated with a carbohydrate stabilizer into tetravalent blends at a target viral concentration per strain and then lyophilized. The purpose of this re-derivation was to enhance the purity of the seed viruses and the traceability of the resulting TDEN vaccine components. Laboratory evaluation and testing in non-human primates of TDEN virus seeds and tetravalent vaccine lots compared with F17/Pre virus seeds and monovalent lots found no major phenotypic or genotypic variations (Eckels K and others, unpublished data).

The vaccines in this study were formulated to have comparable in vitro potency, except that TDEN F19 was planned to contain approximately 10-fold less DENV-4 than TDEN F17 and F17/Pre. Table 1 shows the results of in vitro potency tests for the vaccine treatments performed as previously described.9 The lyophilized placebo contained cell culture medium (EMEM) mixed with an equal volume of stabilizer. After hydration with water for injection (0.5 mL), vaccine or placebo doses having identical appearances were administered subcutaneously into the upper outer triceps/deltoid area.

Study subjects.

Male and female subjects between 18 and 45 years of age were provided the study details, and after informed consent, they were enrolled by staff from the Clinical Trials Center, WRAIR. All were screened for hepatitis B virus surface antigen (HBsAg) and antibodies to hepatitis C virus (HCV) and the human immunodeficiency virus (HIV); they were excluded from participation if positive. Clinically significant laboratory abnormalities at screening, receipt of immune-modifying drugs within 90 days of enrollment, or a history of chronic disease were exclusion criteria. Additional screening tests included a complete blood count (CBC; including white blood cell [WBC] differential and platelet count), blood urea nitrogen (BUN), creatinine, alanine aminotransferase (ALT), and aspartate aminotransferase (AST). Female subjects were of non-childbearing potential or had been abstinent or used adequate contraceptive precautions for 30 days before vaccination, had a negative pregnancy test within 48 hours before vaccination, and agreed to continue such precautions for 60 days after vaccination.

Subjects were not screened for antibodies to DENV. Instead, subjects were retrospectively classified as being DENV-primed or unprimed based on the presence of detectable neutralizing antibodies to any DENV type in a pre-vaccination blood sample (see data analysis below). Proceeding in this manner was considered appropriate, because the precursor vaccine candidate had been safely administered to a small number of DENV primed individuals; such individuals can be at risk for dengue, and they comprise a large proportion of the target population for vaccine prophylaxis.

Safety assessments.

In both study stages, safety was assessed in the following manner. We solicited adverse events (AEs) by asking subjects to record injection site symptoms (injection site pain, redness, and swelling) and general symptoms (fever, fatigue, headache, pain behind the eyes, abdominal pain, nausea, vomiting, muscle ache, joint ache, diffuse rash on the trunk, photophobia, and pruritis) on diary cards for 21 days after each vaccination. Intensities of each AE were scored as grades 1–3, with grade 3 fever defined as an oral body temperature > 39°C (> 102.2°F), grade 3 redness and swelling defined as > 20-mm diameter around the injection site, and all other grade 3 AEs defined as those events preventing normal daily activity.

Investigators conducted active surveillance for AEs of potential cardiac origin occurring after vaccination (chest pain, irregular heart beat or palpitations, shortness of breath, dizziness or loss of consciousness, irregular heart rhythm, pericardial friction rub, and abnormal electrocardiogram [ECG] or elevated troponin I level). If an AE of potential cardiac origin was suspected, the investigator was requested to exclude other (non-vaccine) potential etiologies, and the subject was referred to a cardiologist for definitive assessment. This evaluation was designed to address the theoretical potential for a live DENV vaccine to cause AEs similar to the atypical cardiac manifestations reported after natural DENV infections.12

Subjects were requested to consult an investigator if they developed fever. Subjects were suspected of having dengue if they had (1) fever > 39°C or fever ≥ 38°C measured at least one time on two successive days and (2) at least two of the following signs or symptoms concurrently (nausea, vomiting, headache, eye pain, muscle ache, joint ache, abdominal pain, sore throat, or dengue-like rash). Any subject with suspected dengue underwent additional evaluation (history, physical examination, and clinical laboratory: CBC with WBC differential and platelet count, ALT, and AST) and testing for DENV viremia. Confirmed dengue was a suspected case that was (1) positive for any of the following clinical laboratory abnormalities: absolute neutrophil count (ANC) ≤ 1,000 cells/μL, AST or ALT > 2.5 times the upper limit of normal, hemoconcentration during fever or 1 day after defervescence (peak hematocrit ≥ 1.2 times baseline), or thrombocytopenia < 100,000 cells/μL, and (2) positive for DENV viremia.

On the day of vaccination and again 30 days after each vaccination, subjects were questioned by the investigator about AEs, and a physical examination was performed to evaluate for any dengue-like signs, including rash, hemorrhage (skin, conjunctival, or mucosal), conjunctival injection, hepatomegaly, splenomegaly, or lymphadenopathy. Subjects were also randomly assigned to return for an evaluation on study days 2, 5, 8, or 12 and then again on study days 5, 8, 12, or 14 after each vaccination. Therefore, subjects were assessed on a total of three occasions after each vaccination.

Investigators collected AEs spontaneously reported by subjects that occurred over a 31-day follow-up period after each vaccine or placebo dose. These unsolicited AEs were coded with the use of the Medical Dictionary for Regulatory Activities.13 Investigators also recorded any serious adverse events (SAEs), defined as medically significant events, including those events resulting in hospitalization, disability, or death, throughout the study period.

There were safety laboratory assessments (CBC including WBC, differential and platelet counts, neutrophil count, hematocrit, and ALT and AST) on each vaccination day, two times between days 2 and 14 after vaccination as assigned randomly, and again, 30 days after vaccination. We defined alert laboratory values requiring follow-up as follows: platelet count < 100,000 cells/μL, ANC < 1,000 cells/μL, and ALT or AST > 2.5 times the upper limit of normal.

We systematically evaluated subjects for the presence of dengue viremia during the 31-day period after each vaccine dose in both study stages. Viremia was also measured any time that dengue was suspected. Detection of DENV RNA as a measure of viremia was performed by reverse-transcriptase quantitative polymerase chain reaction (RT-qPCR) using an assay protocol modified from the work by Sadon and others.14

The limit of detection for the RT-qPCR assay was expressed in genome equivalents per milliliter: 6,500 Geq/mL for DENV-1, 160,000 Geq/mL for DENV-2, 1,250 Geq/mL for DENV-3, and 33,000 Geq/mL for DENV-4.

Assays for immune response.

To characterize DENV vaccine immunogenicity, anti-DENV neutralizing antibodies were measured on the day of each vaccination and 1 month after each dose.

A microneutralization assay referred to as MN90 was initially used to measure the dengue antibody titer required to neutralize 90% of the viral input. By reducing the virus input into the neutralization reaction, the assay was refined to estimate a 50% microneutralization endpoint; consequently, all available serum specimens were retested by the qualified MN50 assay as follows. Antibodies to each DENV type were measured at the Pilot Bioproduction Facility, WRAIR, using a 96-well quantitative microneutralization assay (MN50) performed in Vero cells (World Health Organization [WHO], National Institute for Biological Standards and Control [NIBSC]-011038011038) with an initial input of 50 plaque-forming units (PFU) each DENV-2, DENV-3, and DENV-4 and 100 PFU DENV-1. The parental virus strains to be neutralized were DENV-1 WP74, DENV-2 S16803, DENV-3 CH53489, and DENV-4 341750. Seven threefold serial dilutions from 1:3.3 to 1:2,430 were tested per sample. The MN50 titers were automatically processed by an EXCEL spreadsheet, which used a log midpoint linear regression program model to derive the MN50 titer. The MN50 titer is the reciprocal of the serum dilution that neutralizes ≥ 50% of dengue virus, leading to a reduction of 50% of the optical density measured by enzyme-linked immunosorbent assay on fixed cells after 4 days of incubation. Seropositivity was defined as a titer ≥ 1:10.

Data analyses.

This study was exploratory; thus, analyses were descriptive, with no statistical comparisons performed. The primary safety analysis was performed on all enrolled subjects who received at least one vaccine dose (total vaccinated cohort), and the primary immunogenicity analysis was based on the according-to-protocol cohort (ATP; i.e., subjects who met all eligibility criteria, complied with protocol procedures, had no elimination criteria during the study, and had data available for at least one immunogenicity endpoint). Analyses were stratified based on pre-vaccination DENV antibody status (i.e., primed or unprimed). An unprimed subject was defined as having a DENV neutralizing antibody titer < 1:10 to all four DENV serotypes, whereas a primed subject was defined as having a DENV neutralizing antibody titer ≥ 1:10 to any DENV type.

The overall percentages of subjects reporting an AE after vaccine administration (21 days after each vaccination for solicited AEs and 31 days after each vaccination for spontaneously reported symptoms) were tabulated with exact 95% confidence intervals (CIs) by type of AE and intensity (any grade and grade 3). All SAEs occurring during the study were listed for each treatment group. The proportion of subjects with dengue-like physical examination signs detected up to 31 days after each vaccination was tabulated with exact 95% CI.

The proportion of subjects in each group with dengue viremia at each time point within 31 days after vaccination was tabulated after each vaccination. A test for viremia was considered positive if the assay value was greater than or equal to the limit of detection, negative if the assay value was zero, and undetermined if the assay value was > 0 and less than the limit of detection.

We calculated the following immunogenicity parameters by group with seropositivity rate and geometric mean titer (GMT) for each DENV type as well as the tetravalent antibody seroconversion rate. The seropositivity rate was defined as the percentage of subjects with neutralizing antibody titer ≥ 1:10. GMT calculations were performed by taking the antilog of the mean of the log titer transformations, with a value of five given to titers < 1:10. GMTs were calculated with 95% CIs, and seropositivity rates and tetravalent seroconversion rates were calculated with exact 95% CIs. Antibody titers were also summarized by reverse cumulative curves.

Study population.

Eighty-six subjects (twenty-one to twenty-two subjects per group) were enrolled in the study for the first stage starting in April of 2006. All received dose 1 of the candidate vaccine or placebo (Figure 1 shows subject disposition), and 74 subjects (86%) received dose 2. Eleven subjects were withdrawn: one withdrawal was because of an SAE (axonal demyelinating polyneuropathy/bilateral upper and lower extremities 171 days after dose 1 of F19) assessed by the investigator as unrelated to the study treatment. The other 10 subjects moved or were otherwise lost to follow-up. The first stage was completed by June of 2007. In this first stage, 82 subjects were included in the ATP cohort for immunogenicity analysis with the MN90 assay (Figure 1); however, MN50 immunogenicity results were available for only 77 subjects, because the specimens of 5 subjects were consumed in preliminary testing (F17/Pre N = 1, F17 N = 1, F19 N = 3).

Subject disposition. ATP = according to protocol cohort; N = number of subjects.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Subject disposition. ATP = according to protocol cohort; N = number of subjects.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Subject disposition. ATP = according to protocol cohort; N = number of subjects.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Twenty-one subjects (nine subjects from the F17 group and twelve subjects from the F19 group) entered the study's second stage in September of 2007 (Figure 1). These 21 subjects received a third dose of vaccine, and follow-up visits were completed by March of 2008. Of these 21 subjects, MN50 immunogenicity results for all time points (for all three doses) were available for 17 subjects (F17 N = 8, F19 N = 9).

The mean age in the total vaccinated cohort was 34.3 years (median = 35.5 years, range = 20–45 years): 59% were males. Most subjects were either African American (57%) or Caucasian (36%). The above attributes were similar in each group. At baseline, in the ATP cohort with MN50 data available, 14 of 77 subjects (18%) were categorized as primed to DENV, with primed subjects evenly distributed among treatment groups (3–4 primed subjects per group in the ATP cohort). Among the 14 primed subjects in the per-protocol cohort, 11 subjects were primed to all four DENV types, and the other 3 subjects were primed to only one DENV type. Of the 17 subjects in the subset of the ATP cohort who received the third dose and had MN50 data available, there were 4 subjects primed to DENV at baseline: 2 subjects per F17 and F19 groups.

Vaccine safety.

Most subjects (89–100% per group) returned a symptom diary card after vaccination. The incidence of solicited injection site symptoms, all of which were assumed to be causally related to vaccination, is presented in Table 2. Most injection site symptoms were transient, lasted 2 days or less, and mild to moderate in severity; there were few reports of grade 3 symptoms. Injection site symptoms did not seem to increase with dose 2 or in the subset receiving a third dose of TDEN F17 or F19.

The incidence of each solicited general AE is reported per subject considering both doses 1 and 2 (Table 3). The incidence of fever is shown after each dose and both doses. Most reported general symptoms were graded mild or moderate and were transient. Headache was the most frequently reported general symptom (ranging from 33.3% to 54.5% after dose 1 among the four groups and from 16.7% to 37.5% after dose 2) followed by fatigue (ranging from 22.7% to 36.4% after dose 1 among the four groups and from 15% to 25% after dose 2).

As with injection site symptoms, there were no notable differences between groups, including the placebo group, for incidence of any general symptom. This finding was also true for reports of grade 3 general symptoms; these reports were rare, most being reported by one or no subjects per group. In the subset receiving a third dose of TDEN F17 or F19, there were very few reports of general symptoms (Table 4).

During the first study stage, 10–15 subjects in each group (15 [68.2%] subjects in the F17/Pre group, 10 [45.5%] subjects in the F17 group, 15 [71.4%] subjects in the F19 group, and 12 [57.1%] subjects in the placebo group) reported at least one unsolicited symptom during the 31-day follow-up period after each vaccination. Most of the unsolicited AEs reported by DENV vaccine recipients were related to common infections, including bronchitis, a fungal rash, nasopharyngitis, pharyngitis, rhinitis, tonsillitis, or upper respiratory tract infection, gastrointestinal disorders, or respiratory symptoms (cough, nasal congestion, pharyngolaryngeal pain, sinus congestion, or wheezing). Among placebo recipients, most reports were respiratory or musculoskeletal in nature, although disorders of the nervous system were also reported. There was only one report of a grade 3 unsolicited AE that was assessed by the investigator as treatment-related (back pain in a placebo recipient). During the second study stage, 6 of 9 (66.7%) F17 recipients and 3 of 12 (25.0%) F19 recipients reported at least one unsolicited symptom during the 31-day follow-up period for dose 3; only mild pruritis 5 days after vaccination in one subject, based on the history elicited by the investigator (although not recorded in the subject's diary card), was assessed as potentially related to treatment.

For all groups, most abnormal hematological and biochemical levels were also abnormal at baseline. None of the alert values reported after vaccination were associated with suspected dengue. During the study's first stage, there were no alert values reported after doses of F17/Pre or TDEN F17. One F19 vaccine recipient had a serum neutrophil level of 998 cells/μL (alert value defined as < 1,000 cells/mm³) 14 days after dose 1, which returned to normal the next day. One placebo recipient had an AST of 247 U/L (alert value defined as 2.5 times > 50 U/L) 8 days after dose 2, which returned to normal within 4 days. No one in the study's second stage had an alert safety laboratory value.

During study stage 1, investigators examined all subjects during the follow-up visits to find treatment emergent dengue-like signs. They were uncommon and occurred in all treatment groups, including placebo, except for rash/generalized rash, which occurred only in recipients of DENV vaccines (Table 5).

During the study, there were five subjects who had an AE of potential cardiac origin. A cardiologist evaluated all five subjects by history and physical examination, serial ECGs, serial troponin measurements, and in some cases, additional evaluations, including modified stress tests and echocardiograms. None of these events were confirmed as cardiac in origin; none were considered to be caused by the study treatment.

There were four SAEs reported during the entire study: axonal demyelinating polyneuropathy, cerebral bleed secondary to a physical assault, Hodgkin's lymphoma, and post-operative hypertension after surgery required to repair a fracture sustained in a car accident. None of these events were assessed by the investigator as related to vaccination.

DENV viremia.

During study stage 1, DENV-1, DENV-2, and DENV-3 viremia were not detected during the 31-day post-vaccination period; DENV-4 viremia was detected in five subjects (29.4%) in the F17/Pre group and one subject (5.3%) in the F17 group between days 5 and 14 post-vaccination. The magnitude of the DENV-4 viremia ranged from 4.6 to 5.2 log Geq/mL of serum. There were no cases of viremia reported in the F19 or placebo groups. Five of these six subjects with DENV-4 viremia were unprimed before the first vaccination (four subjects in the F17/Pre group and one subject in the F17 group).

There were no alert laboratory findings associated with these six instances of viremia, and there were no symptoms associated with the viremia in the TDEN recipient. However, four of five F17/Pre vaccine recipients with DENV-4 viremia reported symptoms in temporal association with the day that viremia was detected as follows: day 8 post-dose 1 (4.6 log Geq/mL) with grade 1 arthralgia, headache, fatigue, muscle aches, and pain behind the eyes, all lasting 4 days, with rash occurring 1 day later; day 13 post-dose 1 (4.9 log Geq/mL) with fever and symptoms as presented in the case history below; day 14 post-dose 2 viremia (4.6 log Geq/mL) with generalized rash; day 8 post-dose 2 (5.2 log Geq/mL) with grade 2 arthralgia and grade 1 muscle aches for 1 day, grade 2 fatigue for 2 days, and rash and conjunctival injection noted by the investigator on day 13; day 15 post-dose 2 (5.2 log Geq/mL) with no symptoms.

Case history of a febrile illness after DENV vaccine.

Based on the occurrence of fever and other symptoms, dengue was suspected in two subjects, both after dose 1. One subject received F17/Pre vaccine, and the other received placebo. These subjects were evaluated by an investigator with history, physical, and laboratory testing (CBC, ALT/AST, and viremia). Neither case met the clinical and laboratory criteria for confirmed dengue. Nevertheless, the case of the subject who received F17/Pre vaccine is briefly described below, because he was confirmed to have 4.9 log Geq/mL DENV-4 viremia on day 13 after vaccine dose 1.

The affected subject was primed at baseline for all four DENV types. He developed fever and complained of sore throat on day 12, which resolved after 2 days. From day 9 to 16 after dose 1, the subject also reported grades 1–2 headache, nausea, pain behind the eyes, photophobia, rash, pharyngitis, and musculoskeletal pain lasting anywhere from 3 to 12 days.

Immunogenicity.

Immunogenicity was characterized separately for unprimed and primed subjects, because live DENV vaccines can elicit anamnestic multivalent antibody responses after a single dose in individuals having baseline antibody to DENV or other flaviviruses. DENV neutralizing antibody seropositivity rates and GMTs for unprimed subjects with MN50 data available are presented in Tables 6 and 7, and reverse cumulative curves are shown in Figures 3–6.

In unprimed subjects, both TDEN formulations were moderately immunogenic after a single dose; seropositivity rates at 1 month after dose 1 were highest for DENV2 (68.8% F17, 86.7% F19) and somewhat less, although similar, for the other three DENV types (Table 6). Seropositivity rates increased 1 month after dose 2 for all DENV types; responses to DENV2 were again the highest (80.0% F17, 100% F19). Response rates to the other types seemed to be somewhat less, in the range from 66.7% to 83.3%. The rates of seropositivity after doses 1 and 2 of F17/Pre were similar to those rates observed after the TDEN vaccines. No unprimed subject in the placebo group was seropositive after dose 2. In general, there was a slight increase in GMTs for unprimed subjects in all vaccine groups from doses 1 to 2 (Table 7).

Seroconversion rates to each DENV type (i.e., mono-, bi-, tri-, and tetravalent responses) per group and dose are shown in Figure 2. Tetravalent seroconversion rates among the unprimed subjects were modest 1 month after dose 1 for any DENV vaccination (37.5% F17/Pre, 37.5% F17, and 40.0% F19). One month after dose 2, tetravalent rates increased (71.4% F17/Pre, 60.0% F17, and 66.7% F19).

Mono-, bi-, tri-, and tetravalent responses to DENV types in unprimed subjects per group and dose (ATP cohort). Percentages of initially unprimed subjects in each group (F17/Pre, F17, and F19) having seroconverted for none (grey), one (blue), two (green), three (red), or four (orange) DENV types after each dose of the candidate vaccine are shown. Blood samples were taken from subjects 1 month after each dose.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Mono-, bi-, tri-, and tetravalent responses to DENV types in unprimed subjects per group and dose (ATP cohort). Percentages of initially unprimed subjects in each group (F17/Pre, F17, and F19) having seroconverted for none (grey), one (blue), two (green), three (red), or four (orange) DENV types after each dose of the candidate vaccine are shown. Blood samples were taken from subjects 1 month after each dose.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Mono-, bi-, tri-, and tetravalent responses to DENV types in unprimed subjects per group and dose (ATP cohort). Percentages of initially unprimed subjects in each group (F17/Pre, F17, and F19) having seroconverted for none (grey), one (blue), two (green), three (red), or four (orange) DENV types after each dose of the candidate vaccine are shown. Blood samples were taken from subjects 1 month after each dose.

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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In unprimed subjects, acknowledging the small groups sizes, there were no striking differences among the reverse cumulative curves of neutralizing antibody titers by DENV treatment after dose 2 for any DENV type (Figures 3–6).

Reverse cumulative curves of DENV-1 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-1 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-1 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-2 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-2 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-2 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-3 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-3 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-3 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

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Reverse cumulative curves of DENV-4 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-4 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Reverse cumulative curves of DENV-4 neutralizing antibody titers 1 month after dose 1 and dose 2 for each vaccine group for unprimed subjects (ATP cohort for immunogenicity).

Citation: The American Society of Tropical Medicine and Hygiene 88, 1; 10.4269/ajtmh.2012.12-0361

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Among the 14 primed subjects in the per-protocol immunogenicity cohort with MN50 data available (3–4 subjects per group), the tetravalent rate was 100% 1 month after dose 2 (data not shown), with high GMTs to each DENV type regardless of DENV treatment.

Individual antibody titers of subjects in study stage 2 who had MN50 data available at 1 month post-dose 2 and pre- and post-dose 3 visits are provided in Table 8. The tetravalent response rates before and 1 month after dose 3 (stage 2) in unprimed subjects were 16.7% and 66.7% in six F17 recipients and 28.6% and 57.1% in seven F19 recipients. Among the primed subjects who were in study stage 2 (two subjects in F17 and two subjects in F19), the tetravalent rate was 100% on the day of dose 3 and 1 month later. There was no important change in antibody level to any DENV type for any subject.