70E-18 26 54% 21,28 A,B 5 Dihydrolipoyllysine-residue succinyltransferase sucB CBU_1398 gi|29654691 45908 5.54 MALDI-TOF 100 0.00027 16 34% 21,28 A 6 Fructose-1,6-bisphosphate aldolase fbaA CBU_1778 gi|29655066 39793 5.41 MALDI-TOF 190 2.70E-13 16 48% 21,28 A,B 7 S-adenosylmethionine Synthetase
metK CBU_2030 gi|29655311 43150 5.55 MALDI-TOF 153 1.40E-09 20 50% – A,B 8 3-oxoacyl-[acyl-carrier-protein] synthase 2 fabF CBU_0497 gi|29653839 44275 5.49 MALDI-TOF 160 2.70E-10 20 58% – A 9 Elongation factor Tu tuf2 CBU_0236 gi|29653588 43613 5.32 MALDI-TOF 285 8.60E-23 29 76% 28 A,B 10 Glutamine synthetase glnA CBU_0503 gi|29653845 39876 5.33 MALDI-TOF 122 1.7e-06 15 44% – A 11 Malate dehydrogenase mdh CBU_1241 gi|29654544 4SC-202 ic50 35732 5.07 MALDI-TOF 136 6.80E-08 19 50% 21,28 A 12 34 kDa outer membrane JQ-EZ-05 supplier protein ybgF – gi|30025849 33641 5.67 MALDI-TOF 92 0.0019 8 28% 21,28 A 13 (2R)-phospho-3-sulfolactate synthase comA CBU_1954 gi|29655237 33383 5.38 MALDI-TOF 146 6.80E-09 16 52% 28 A 14 Inorganic diphosphatase ppa CBU_0628
gi|29653966 19642 5.2 ESI-MS/MS 323 2.1e-26 7 36% 28 – 15 LSU ribosomal protein L12P (L7/L12) rplL CBU_0229 COXBURSA gi|29653581 13240 4.71 ESI-MS/MS 210 4.2e-15 6 48% – A,B 16 30S ribosomal protein S2 rpsB 331_A1545 gi|161831161 35410 8.88 MALDI-TOF 100 0.00027 15 48% 28 – 17 Peptidyl-prolyl cis-trans isomerase Mip mip CBU_0630 gi|29653968 Lenvatinib 25501 9.8 MALDI-TOF 133 6.10E-07 9 57% 14,21,28 – 18 27 kDa outer membrane protein com1 – gi|11935138 26739 9.23 MALDI-TOF 95 0.00078 7 42% 14,21,28
– 19 Acute disease antigen A adaA CBU_0952 gi|29654269 25935 8.67 MALDI-TOF 110 2.70E-05 15 38% – B 20 Putative Non-specific serine/threonine protein kinase outer membrane Skp ompH CBU_0612 gi|29653950 18812 9.71 ESI-MS/MS 429 4.3e-37 5 28% 14,21,28 – Serological analysis of the recombinant seroreactive proteins with Q fever patient sera Twenty genes encoding the seroreactive proteins were amplified (Additional file 1: Table S1) and cloned into the pET32a/pQE30 plasmid. The 19 recombinant proteins were purified by Ni-NTA agarose and analyzed by sodium dodecylsulfate polyacrylamide gel electrophoresis (SDS-PAGE). Then they were used to fabricate a protein microarray. The protein microarray was probed with 56 sera from patients with acute Q fever and 25 sera from healthy persons (normal sera). The average FI value of the proteins probed with acute early, late or convalescent Q fever patient sera were significantly higher compared with that probed with the normal sera (P < 0.05) The average FI values of the proteins probed with acute late Q fever patient sera were significantly higher than acute early or convalescent Q fever patient sera (P < 0.05). The protein was considered to be seroreactive if its average FI probed with the patient sera were higher than the mean FI plus twice the standard deviation probed with normal sera (Additional file 2: Table S2).