| Literature DB >> 23144798 |
Francesca Micoli1, Simona Rondini, Massimiliano Gavini, Luisa Lanzilao, Donata Medaglini, Allan Saul, Laura B Martin.
Abstract
Enteric fevers remain a common and serious disease, affecting mainlyEntities:
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Year: 2012 PMID: 23144798 PMCID: PMC3492368 DOI: 10.1371/journal.pone.0047039
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240
Figure 1Structure of S. Paratyphi A O-antigen chain linked to the core region [22]; [23].
Reductive amination of O:2-KDO with ADH is pH dependent and temperature independent.
| Buffer | Temperature | % activated O:2 |
| Sodium acetate pH 4.5 | 30°C | 65.8 |
| Sodium acetate pH 4.5 | 50°C | 65.4 |
| Sodium acetate pH 4.5 | 60°C | 68.3 |
| MES pH 6.0 | 30°C | 43.9 |
| Phosphate pH 8.0 | 30°C | 26.2 |
Figure 2O:2-ADH-SIDEA-CRM197 conjugation scheme.
Same reaction was also performed with the shorter linker CDH instead of ADH.
Reproducibility of O:2-ADH and O:2-ADH-SIDEA intermediates.
| Sample | % Sugar recovery(average ± SD) | % Activated O:2 chainwith ADH (average ±SD) | % Free/totalhydrazide groups | % Derivatized withSIDEA (average ± SD) | % Free/total active ester groups |
| O:2-ADH | 76.0±4.4 | 80±0.4 | <5 | – | – |
| O:2-ADH-SIDEA | 84.8±7.9 | – | – | 81.9±2.2 | <10 |
Figure 3SDS-PAGE analysis of conjugation mixtures in comparison to unconjugated CRM197.
Lane 1: marker, lane 2: CRM197, lane 3: O:2-(CDAP)ADH-CRM197 conjugation mixture, lane 4: O:2-(EDAC)ADH-CRM197 conjugation mixture, lane 5: O:2-ADH-SIDEA-CRM197 conjugation mixture, lane 6: O:2-CDH-SIDEA-CRM197 conjugation mixture, lane 7: O:2-SIDEA-CRM197 conjugation mixture. Ten µg of protein were loaded per conjugation mixture, 5 µg for CRM197.
Figure 4Gel filtration profiles on Sephacryl S-300 HR column (1.6×90
cm) of O:2-ADH-SIDEA-CRM Elution with 50 mM NaH2PO4, 0.15 M NaCl, pH 7.2 at a flow rate of 0.5 mL/min. Arrows indicate the fractions pooled to generate purified conjugate.
Characterization of the conjugates used in the immunogenicity study in mice.
| Conjugate | Total sugar, µg/mL | Total protein, µg/mL | wt/wt ratio O:2 to CRM197 | Kd (HPLC-SEC) |
| O:2-(CDAP)ADH-CRM197 | 32.88 | 62.98 | 0.52 | 0.44 |
| O:2-CDH-SIDEA-CRM197 | 82.82 | 36.67 | 2.26 | 0.40 |
| O:2-ADH-SIDEA-CRM197 | 51.54 | 29.56 | 1.74 | 0.39 |
| O:2-(EDAC)ADH-CRM197 | 50.19 | 31.31 | 1.60 | 0.52 |
| O:2 | 0.55 | |||
| CRM197 | 0.69 |
Figure 5HPLC-SEC analysis of A) O:2; B) O:2-ADH; C) O:2-ADH-SIDEA (RI detection).
Samples run on TosoHaas TSK gel 3000 PWXL column; eluent: 0.1 M NaH2PO4, 0.1 M NaCl, 5% CH3CN, pH 7.2; flow rate: 0.5 mL/min. Column void volume: 10.85 min.; total volume: 23.54 min. O:2 molecular weight distribution remains unchanged during the O:2 derivatization steps with ADH and SIDEA (all the samples have Kd of 0.17).
O:2 chain sugar composition remains unchanged during conjugation steps to produce O:2-ADH-SIDEA-CRM197.
| Sugar composition, molar ratio | ||||
| by 1H NMR | by HPAEC-PAD | |||
| Sample | Par/Rha | Man/Rha | Gal/Rha | Glc/Rha |
| Underivatized O:2 | 1.06 | 1.07 | 1.05 | 0.74 |
| O:2-ADH | 1.08 | 1.05 | 0.99 | 0.73 |
| O:2-ADH-SIDEA | 1.08 | 1.05 | 0.98 | 0.83 |
| O:2-ADH-SIDEA-CRM197 | 1.05 | 1.04 | 1.07 | 0.83 |
Figure 61H NMR spectra of A) O:2 (68% OAc); B) O:2-ADH (70% OAc); C) O:2-ADH-SIDEA (68% OAc); D) O:2-ADH-SIDEA-CRM197 (67% OAc).
O-acetylation level quantified by comparing acetate (released after treatment with NaOD, at 1.91 ppm) and Rha-H6 peaks at 1.40 ppm, and expressed as molar % of O-acetyl with respect to OAg chain repeating units (being Rha present only in the OAg chain, at one sugar per repeating unit). O-acetylation level is maintained at the same level after conjugation.
Figure 7HPLC-SEC profiles (fluorescence emission detection) of O:2-ADH-SIDEA-CRM197 (dotted line; 28.7 µg/mL of protein; Kd of 0.39) in comparison to free CRM197 (dashed line; 50 mg/mL; Kd of 0.69) and free O:2 (solid line; 1 mg/mL of sugar; Kd of 0.55).
80 µL of each samples run on TosoHaas TSK gel 6000+5000 PW columns; eluent: 0.1 M NaH2PO4, 0.1 M NaCl, 5% CH3CN, pH 7.2; flow rate: 0.5 mL/min. Column void volume: 23.65 min.; total volume: 49.07 min. Free O:2 is not detected by fluorescence emission.
Characterization of conjugates after purification on Sephacryl S-300 HR column.
| Conjugate | Total sugar, µg/mL | Total protein, µg/mL | Wt/wt ratio O:2 toCRM197 | Kd (HPLC-SEC) |
| O:2-ADH-SIDEA-CRM197 | 51.54 | 29.56 | 1.74 | 0.39 |
| O:2-SIDEA-CRM197 | 108.6 | 52.8 | 2.06 | 0.38 |
| O:2-(TNBS)ADH-SIDEA-CRM197 | 54.8 | 23.7 | 2.31 | 0.44 |
Figure 8SDS-PAGE analysis.
Lane 1: marker, lane 2: CRM197 (5 µg), lane 3: conjugation mixture of O:2(TNBS)-SIDEA + CRM197 (10 µg of protein), lane 4 conjugation mixture of O:2(TNBS)-ADH-SIDEA + CRM197(10 µg of protein).
Figure 9Anti-O:2 IgG (panel A) and Anti-CRM197 (panel B) serum IgG ELISA units detected in sera of CD-1 mice immunized with O:2-conjugates and unconjugated O:2.
Mice were immunized three times at two week-intervals with the indicated doses of material. Mice were bled and sera collected on the indicated days. Individual animals are represented by the scatter plots; bars represent the group geometric mean.
Figure 10SBA assay performed with pooled mouse sera from different immunization groups and CVD1901.
Data are presented as percentage of CFU recovered in test sera with active BRC (and in control serum with inactive BRC) compared with CFU present in negative control, per anti-O:2 ELISA antibody unit of each serum pool.