Jussi Mertsola
University of Texas Southwestern Medical Center
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Featured researches published by Jussi Mertsola.
Antimicrobial Agents and Chemotherapy | 1990
Xavier Sáez-Llorens; Octavio Ramilo; Mahmoud M. Mustafa; Jussi Mertsola; C de Alba; Eric J. Hansen; George H. McCracken
Pentoxifylline has been shown to decrease endotoxin-induced tumor necrosis factor alpha production and reverse the inflammatory actions of interleukin-1 (IL-1) and tumor necrosis factor on leukocyte function. Because of the potential role of this cytokine-leukocyte interaction in the pathogenesis of bacterial meningitis, we investigated the ability of pentoxifylline to modulate meningeal inflammation in the rabbit meningitis model. Pentoxifylline treatment (initially an intravenous injection of 20 mg/kg followed by 6 mg/kg per h) started 20 min before intracisternal injection of 20 ng of Haemophilus influenzae type b lipooligosaccharide (endotoxin) reduced significantly concentrations in cerebrospinal fluid of leukocytes (P less than 0.0001), protein (P less than 0.001), and lactate (P less than 0.001) during the 9-h infusion compared with values in intravenous-saline-treated rabbits. When pentoxifylline was given 1 h after H. influenzae type b endotoxin, the mean peak lactate and leukocyte concentrations in cerebrospinal fluid were significantly lower than those in control animals. Pentoxifylline also significantly decreased lactate and protein concentrations (P less than 0.05) and tended to diminish leukocyte counts (P = 0.08) compared with results in control animals after antibiotic-induced release of endotoxin in animals with H. influenzae meningitis. In this regard, dexamethasone was superior to pentoxifylline and no synergism was observed when the drugs were combined. Additionally, pentoxifylline attenuated meningeal inflammatory changes induced by intracisternal inoculation of 10 ng of rabbit recombinant IL-1 beta compared with results in either dexamethasone- or saline-treated animals. We conclude that pentoxifylline is effective in this animal model in modulating the meningeal inflammatory response following intracisternal inoculation of H. influenzae type b endotoxin or organisms or rabbit recombinant IL-1beta.
Molecular Microbiology | 1991
Leslie D. Cope; Ram Yogev; Jussi Mertsola; Jo L. Latimer; M. S. Hanson; George H. McCracken; Eric J. Hansen
A wild‐type Haemophilus influenzae type b (Hib) genomic DNA library was constructed in the plasmid shuttle vector pGJB103. A virulence‐deficient lipooligosaccharide (LOS) mutant of Hib was used as a recipient for genetic transformation to screen this Hib genomic DNA library for genes involved in LOS expression. A recombinant plasmid containing a 7.8 kb Pstl fragment of Hib DNA was shown to transform this LOS mutant to reactivity with a monoclonal antibody (mAb) specific for a wild‐type LOS epitope. Transformation of two different virulence‐deficient LOS mutants with a 4.4kb BglII fragment of this recombinant plasmid yielded transformants which expressed LOS that bound the wild‐type LOS‐specific mAb and yielded profiles in sodium dodecyl sulphate/polyacrylamide gradient gel electrophoresis different from those of the original LOS mutants. These transformants with structurally altered LOS molecules also exhibited increased virulence in an animal model for invasive Hib disease. The virulence‐transforming ability was further localized to a 1.8kb BglII‐AlwNI fragment of the Hib DNA insert. Nucleotide sequence analysis indicated the presence of a single large open reading frame within this fragment. This open reading frame contained 19 consecutive repeats of the tetramer CAAT near the 5’end. Linker insertion mutagenesis was used to demonstrate directly the involvement of this open reading frame in both LOS biosynthesis and virulence expression by Hib.
Journal of Immunological Methods | 1989
Jussi Mertsola; Octavio Ramilo; Xavier Sáez-Llorens; M. S. Hanson; George H. McCracken; Eric J. Hansen
A monoclonal antibody (MAb)-based enzyme immunoassay was developed for detection of Haemophilus influenzae type b (Hib) lipooligosaccharides (LOS). The high affinity of polymyxin B for lipid A was used to bind the Hib LOS to microtiter wells. The immobilized LOS was detected with MAbs directed against the oligosaccharide component of Hib endotoxin. Hib LOS concentrations were measured in in vitro samples and in cerebrospinal fluid (CSF) sample obtained from rabbits with experimental Hib meningitis. The sensitivity of the assay was 1 ng LOS/ml sample and the results obtained with this assay correlated significantly with those obtained with the standard Limulus amebocyte lysate assay. This new assay provides a method for specific detection of Hib LOS in CSF samples and in aqueous laboratory fluids. This general methodology should also be useful for experimental research involving specific LPS/LOS molecules.
Journal of Experimental Medicine | 1990
Octavio Ramilo; Xavier Sáez-Llorens; Jussi Mertsola; Hamid Jafari; Kurt Olsen; Eric J. Hansen; Masaru Yoshinaga; Susumu Ohkawara; Hideo Nariuchi; George H. McCracken
The Journal of Infectious Diseases | 1989
Mahmoud M. Mustafa; Octavio Ramilo; Jussi Mertsola; Richard C. Risser; Bruce Beutler; Eric J. Hansen; George H. McCracken
The Journal of Infectious Diseases | 1989
Mahmoud M. Mustafa; Jussi Mertsola; Octavio Ramilo; Xavier Sáez-Llorens; Richard C. Risser; George H. McCracken
JAMA Pediatrics | 1990
Octavio Ramilo; Mahmoud M. Mustafa; John Porter; Xavier Sáez Llorens; Jussi Mertsola; Kurt Olsen; James P. Luby; Bruce Beutler; George H. McCracken
JAMA Pediatrics | 1991
Jussi Mertsola; William A. Kennedy; David C. Waagner; Xavier Sáez-Llorens; Kurt Olsen; Eric J. Hansen; George H. McCracken
Pediatric Infectious Disease Journal | 1989
Jussi Mertsola; Octavio Ramilo; Mahmoud M. Mustafa; Xavier Sáez-Llorens; Eric J. Hansen; George H. McCracken
Infection and Immunity | 1990
Leslie D. Cope; Ram Yogev; Jussi Mertsola; J C Argyle; George H. McCracken; Eric J. Hansen