title

1. title CD4+ T-cell responses among adults and young children in response to Streptococcuspneumoniae and Haemophilus influenzae vaccine candidate protein antigens.

2. 1.Introduction • Adults and children are frequently affected by infections caused by Steptococcus pneumoniae(Spn) and non-typeable Haemophilus influenzae(NTHi) , accounting for an increased incidence of pneumonia,invasive Spn disease ,acute sinusits and acute otitis media[1-3]. • Among the vaccine candidates ,pneumococcal surface protein A(PspA),PhtD and PhtE,a choiline binding protein-PcpA,a murein hydrolase (-LytB)and a non-toxic pneumolysin derivative PlyD1,have emerged as most likely to proceed to clinical trials in humans[7-11].

3. CD4+T lymphocytes have been shown to be important for protective immumnity against Spn and NTHi infections inboth adult and mice [16-18].However,there are no date that demonstrate the nature of CD4+T lymphocyte responses to Sgn and NTHi among younger children ,and their comparative analysis with adults. In this study we characterized and compared circulating antigen-specific CD4+T lymphocyte populations responsive to six Spn and twoNTHi antigens in adults and young children.

4. 2.Materials and methods 2.1 Subjects and samples Eleven healthy adults (five females and six males; median age 32.5 years ) and 17 young children( 6 months to three years old) None of the subjects had experienced invasive Spn infections or lobar pneumonia.PBMCs were isolated using a Ficoll gradient according to the manufacturer's instruction (GE Healthcare) and then washed with 1×phosphate buffered saline (PBS),re-suspended at a concentration of 1×107 cells/ml in cell recovery freezing media (Gibco) and frozen in liquid nitrogen until used.

5. 2.2 Antigens and antibodies • Pneumococcal protein antigens that were used for T-cell stimulation included : PspA(EF5668) PhtD , PhtE LytB PcpA PlyD1 • Antibodies: CD3 Qdot 605 (cione UCHT1,Invitogen) CD3Qdot 605 anti-CD4 APC Alex Flor 750 (clone RPAT4, eBiosciences) PE-Cy5 anti-CD69(cloneFN50, BD biosciences)...

6. 2.3PBMC stimulation for detection of intracellular cytokine • Thawing frozen PBMCs • Counting cells • Resting overnight in complete culture media in 24-well plates • Stimulating • Counting again and stimulating • Incubating ,after 2 h golgi transport inhibitors were added to preserve cytokines intracellularly and incubated for an additional 4 h.anti -CD28 and anti-CD49d antibodies were also added to provide co -stimulation and enhance the detection of antigen specific response as described earlier [26,27]

7. 2.4. surface and intracellular staining for flow cytometric analysis. • Transfering to 96-well V-bottom and washing • Incubating • Permeabilizing • Intracellular staing • Furtherwashing • Collecting 0.2-1 ×106 events for each sample and analyzing with FLOW JO (Tree Star )software.

8. 2.5. Cytometric bead array (CBA )for detection of secreted cytokines • For CBA assay, PBMCs were thawed and rested overnight as described previously before stimulating them with either 1µg/ml • of individual antigens or SEB for 18-20h. After stimulation, super natants were collected and cytokines were meansured using a CBA kit for TH -1and TH -2 cytokine detection (BD Biosciences )as described by the manufacturer.

9. Acquisition template provided by BD was used to acquire cytometric beads on a LSRⅡ flow cytometer and date was analyzed using BD FACSDIVA software and Flowjo.Standard graphs were plotted and unknown sample values wre extrapalates on linear regression plots with GraphPAD Prism 5 software.

10. 2.6.Statistical analysis • We used a rank based procedure, related to the Friedman blocked rank design, to determine those antigens with consistently high or low responses to specific cytokines. • To assess the statistical significance of the average ranks a bootstrap procedure was used.

11. 3.Results

13. 3.1.CD4 + T-cell responses to spn and NTHi antigens in adults • The IL-4 IL-10and IL-13 responses were generally lower than IL-2 and IFNγ responses.No IL-17 responses were detected in adult (data not show) • In addition,all cytokines exhibited significantly non-hemogeneous responses with respect to antigen exposures.

14. 3.2 Characteristics of CD4+T-cell responses to spn and NTHi protein antigens in very young children • Overall,compared with negative controls, IL-2 and IFNγ producing cells exhibited significantly higher responses to vaccine antigen stimulations in young children. • IL-17 producing CD4+ Th-cell were infrequent and were present only in a few children（data not show)

15. 3.3Divergence of CD4+ T-cell responses to Spn and NTHi protein antigens in young children versus adults. Adults had vaccine antigen-specifc Th1 and Th2 cells responsive to all antigens evaluated whereas young children had significant numbers of vaccine antigen-specific CD4+ T-cell producing IL-2

18. 3.4 Memory phenotypes of Spn and NTHi specific CD4+ T-cells among very young children and adults • Vaccine antigen-specificCD4+ T-cell populations in adults were largely of effector(TEM)and/or central memory (TCM)phenotypes as denfined by CD45RA-CCR7+orCD45RA-aCCRA-respectively; however among young children antigen-specific IL-2 producingCD4+ T-cells demonstrated CD45RA+ expression (non-memory cells)

20. Therefore,vaccination with the studied antigens would likely to boost higher CD4 T-cell responses among adults,whereas young children have a more limited response.

21. 4.Discussion • . Adults,who have a more mature immune system and who have more accumulated natural exposures to Spn and NTHi,had significantly higher antigen-specific CD4+T-cells compared to young children .In fact,in adults all tested vaccine candidate antigens stimulatedCD4+ T-cell responses,predominantly with a Th-1profile

22. In conclusion , this report demonstrates the frequencies of Spn and NTHi antigen specific CD4+ T-cells among adults compared to young children following natural exposure to the bacteria. • Identified aspects contributing to the divergence between the age populations should represent target areas for evaluation of immune-response enhancing approaches.

23. THE END!