M. Vanstaden et al., DETECTION OF MYCOBACTERIUM-TUBERCULOSIS IN SERUM SAMPLES USING THE POLYMERASE-CHAIN-REACTION, The Journal of infection, 36(3), 1998, pp. 273-277
Conventional methods for the diagnosis of Mycobacterium tuberculosis i
nfections have serious limitations. To determine whether amplification
of M. tuberculosis DNA in serum by the polymerase chain reaction (PCR
) might be a useful additional diagnostic tool, we tested 329 clinical
specimens using primers specific for the IS6110 insertion sequence of
the M. tuberculosis complex. The samples consisted of 30 serum sample
s from healthy controls, 114 serum samples from patients with diagnose
s other than tuberculosis (including immunosuppressive disorders), 59
samples from patients with a clinical picture suggestive of tuberculos
is, and 78 serum samples from patients with proven M. tuberculosis inf
ection. Both serum, and representative samples from anatomical regions
suspected of being infected, were collected from a further 48 patient
s for comparison with serum PCR. Serum PCR identified 72/78 (92%; 95%
confidence interval CI: 84%-97%) patients with proven tuberculosis, an
d 49/59 (83%; 95% CI: 71%-92%) patients with suspected tuberculosis. I
n the group of patients with other diagnoses, 30/114 (26%; 95% CI: 18%
-34%) tested positive, while none of the specimens from the healthy co
ntrol group were positive (95% CI: 0%-12%). Serum PCR results also com
pared favourably with other clinical specimens obtained from the same
patient. Serum PCR can, therefore, be a useful additional technique fo
r the early diagnosis of M. tuberculosis infection, but it does not ne
cessarily indicate active infection.