All Posts Tagged With: "B. quintana"

Link: http://eutils.ncbi.nlm.nih.gov/entrez/eutils/elink.fcgi?dbfrom=pubmed&id=21289156&retmode=ref&cmd=prlinks

Excerpt:

In this study we compared some common Bartonella culturing methodologies
using four diverse species causing human illnesses. Based on a review of the
literature, we focused on three major inconsistencies between protocols:
base media, cell co-culture and temperature. Our data showed that B. tamiae
demonstrated temperature-dependent growth limitations between common
culturing conditions only 2 degrees C apart. Additionally, growth of B.
quintana was significantly enhanced by the presence of mammalian cell
co-culture within mammalian culture conditions, however when the media was
modified to incorporate insect culture-based media, co-culturing with
mammalian cells was no longer needed. In this study, we were able to
overcome these temperature and cell dependent limitations and accommodate
all of the strains tested by combining mammalian culture-based media with
insect culture-based media.

Excerpt:

A gram-negative, rod-shaped microorganism was detected in a
69-year-old man suffering from chronic back pain but otherwise
exhibiting no signs of infection.
The bacterium could not be identified using any routine
diagnostic modality. A research use only application utilizing
PCR and Mass Spectrometry was performed on nucleic acid extracted
from the tissue sample. These studies resulted in the implication
of Bartonella quintana as the underlying cause of the infection.
B.
quintana is not a well-known cause of an abdominal aortic mycotic
aneurysm. This article will discuss the B. quintana infection,
its diagnosis and treatment, and reinforce the potential of B.
quintana as a possible etiology in mycotic aneurysms that show no
apparent indications of infection. It will also explore the
potential use of polymerase chain reaction detected by
electrospray ionization mass spectrometry (PCR/ESI-MS) to help
identify B. quintana in a situation where other conventional
methods prove non-informative.

Full article: http://www.lymeneteurope.org/forum/viewtopic.php?f=7&t=1336#p9502

Excerpt:

Abstract
Using PCR in conjunction with pre-enrichment culture, we detected Bartonella henselae and B. vinsonii subspecies berkhoffii in the blood of 14 immunocompetent persons who had frequent animal contact and arthropod exposure.

Attempts to isolate Bartonella sp. from immunocompetent persons with serologic, pathologic, or molecular evidence of infection are often unsuccessful; several investigators have indicated that Bartonella isolation methods need to be improved (1–4). By combining PCR and pre-enrichment culture, we detected B. henselae and B. vinsonii subspecies berkhoffii infection in the blood of immunocompetent persons who had arthropod and occupational animal exposure

The Study

From November 2004 through June 2005, blood and serum samples from 42 persons were tested, and 14 completed a questionnaire, approved by the North Carolina State University Institutional Review Board. Age, sex, animal contact, history of bites, environment, outdoor activity, arthropod contact, travel, and medical history were surveyed. Bacterial isolation, PCR amplification, and cloning were performed by using previously described methods (5–7). Each blood sample was tested by PCR after direct DNA extraction, pre-enrichment culture for at least 7 days, and subculture onto a blood agar plate (Figure). An uninoculated, pre-enrichment culture was processed simultaneously as a control. Methods used for DNA extraction and conventional and real-time PCR targeting of the Bartonella 16S-23S intergenic spacer (ITS) region and heme-binding protein (Pap31) gene have been described (7,8). Conventional PCR amplicons were cloned with the pGEM-T Easy Vector System (Promega, Madison, WI, USA); sequencing was performed by Davis Sequencing, Inc. (Davis, CA, USA). Sequences were aligned and compared with GenBank sequences with AlignX software (Vector NTI Suite 6.0 (InforMax, Inc., Bethesda, MD, USA) (7,8). B. vinsonii subsp. berkhoffii, B. henselae, and B. quintana antibodies were determined by using a modification of a previously described immunofluorescence antibody assay (IFA) procedure (9

Study participants included 12 women and 2 men, ranging in age from 30 to 53 years; all of them reported occupational animal contact for >10 years (Table). Most had daily contact with cats (13 persons) and dogs (12 persons). All participants reported animal bites or scratches (primarily from cats) and arthropod exposure, including fleas, ticks, biting flies, mosquitoes, lice, mites, or chiggers. All participants reported intermittent or chronic clinical symptoms, including fatigue, arthralgia, myalgia, headache, memory loss, ataxia, and paresthesia (Table). Illness was most frequently mild to moderate in severity, with a waxing and waning course, and all but 2 persons could perform occupational activities. Of the 14 participants, 9 had been evaluated by a cardiologist, 8 each by an infectious disease physician or a neurologist, and 5 each by an internist or a rheumatologist. Eleven participants had received antimicrobial drugs.