Chemistry: molecular biology and microbiology – Measuring or testing process involving enzymes or... – Involving antigen-antibody binding – specific binding protein...
Reexamination Certificate
1999-09-16
2004-11-30
Portner, Ginny (Department: 1645)
Chemistry: molecular biology and microbiology
Measuring or testing process involving enzymes or...
Involving antigen-antibody binding, specific binding protein...
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Reexamination Certificate
active
06824997
ABSTRACT:
BRIEF DESCRIPTION OF THE INVENTION
The present invention relates to a specific and sensitive immunochromatographic (“ICT”) assay, performable within about 15 minutes, for the detection of
Streptococcus pneumoniae
in a bodily fluid, such as urine or cerebrospinal fluid, of a patient showing clinical signs of an infection caused by
S. pneumoniae.
BACKGROUND OF THE INVENTION
Streptococcus pneumoniae
(“
S. pneumoniae
”) is a leading causative organism of pneumonia-type illnesses and other lower respiratory tract infections such as bronchitis, as well as of upper respiratory tract infections, including infectious otitis media and sinusitis and of disseminated invasive infections, including bacteremia and meningitis. When not properly diagnosed and treated,
S. pneumoniae
pneumonic infection may lead to any of pericarditis, empyema, purpura fulmiran, endocarditis or at least one type of arthritis, where
S. pneumoniae
is the causative organism in each instance. Such pneumonic infection is also often a precursor of bacteremia or meningitis. To now, it nevertheless is common for pneumonia arising from
S. pneumoniae
to be diagnosed and treated somewhat empirically.
To a significant extent, this is because the tests presently available for the detection of
S. pneumoniae
are either (1) time consuming, labor intensive and in need of instrumental assistance for reading results, or (2) lacking in sensitivity and/or specificity. Because of problems associated with lack of sensitivity and/or specificity, e.g., physicians tend toward conservatively prescribing expensive, broad spectrum antibiotics for patients with pneumonia-type respiratory infections in lieu of prescribing a less expensive antibiotic specific to
S. pneumoniae
where it would adequately cure the infection. This and other liberal prescribing of broad spectrum antibiotics is, of course, a major cause of today's well-publicized medical crisis consequent from the increasing resistance of many types of infectious bacteria to previously highly efficacious antibiotics. This crisis and the potential untoward consequences for at least some patients of empirical diagnosis and treatment are among many reasons why a reliable and rapid assay for detecting
S. pneumoniae
in human body fluids is needed.
Pneumonia caused by
S. pneumoniae
is a serious disease, estimated to occur at the rate of one to five cases per 1,000 persons per year in the United States alone. Depending upon the age and state of health (based on unrelated factors) of patients infected with
S. pneumoniae
-caused pneumonia, the disease has a mortality rate of between 4 percent and 30 percent of infected patients.
The most time-honored methods of attempting to diagnose
S. pneumoniae
-caused diseases, and especially pneumonia, involve the Gram stain and culture of expectorated sputum of patients suspected of harboring the disease, followed by biochemical identification methods. This procedure requires in the order of one to four days from start to finish. It has proved to be an unsatisfactory diagnostic tool because (1) other bacteria present in the patient's saliva often overgrow the sputum culture, and (2)
S. pneumoniae
frequently is present in the human upper respiratory tract even when no sign of disease attributable to this bacterium is present in the individual. For example, it is estimated that some 30 percent of U.S. children are habitual carriers of
S. pneumoniae
. Adults, too may become colonized by
S. pneumoniae
without themselves entering a disease state. The carriage rates of the organism by both children and adults increase with crowding conditions and during winter months.
Co-agglutination, latex particle agglutination and counter-immunoelectrophoresis methods for detecting the polysaccharide capsular antigens of
S. pneumoniae
in sputum specimens have been developed and are rapid, but they have not been shown to exhibit reliable sensitivity or specificity, probably because there are some 83 serotypes of
S. pneunoniae
, each of which may vary in immunogenicity and in other respects. The commercial polyvalent anti-serum developed and used for these tests contains antibodies to all 83 of the
S. pneumoniae
serotype antigens, but it nevertheless may fail to detect the less immunogenic antigen serotypes. This polyvalent antiserum also has shown cross-reactivity with other streptococci and some other infectious bacteria, e.g.,
Haemophilus influenzae
. Hence both false-negative and false-positive reactions may occur randomly when these tests are used on sputum samples.
Several enzyme-inmmunoassays (“EIA”) have been developed which are based on detection of the pneumococcal C-polysaccharide antigen that has been found to be present in the pneumococcal cell wall of all of the
S. pneumoniae
serotypes. See, e.g., Parkinson, A. J., Rabiego, M. E., Sepulveda, C., Davidson, M. and Johnson, C., 30
J. Clin. Microbiol
. 318-322 (1992). This C-polysaccharide antigen is a phosphocholine-containing polysaccharide derived from teichoic acid. These EIA assays are of acceptable specificity and sensitivity even though most often performed on sputum samples. Each such assay, however, requires two to three hours performance time after sample collection as well as the use of instrumentation normally available primarily in clinical laboratories. In addition, these assays need to be run by, or under close supervision of, trained personnel.
Reliance upon sputum samples to diagnose
S. pneumoniae
infections is frequently less than satisfactory in achieving a diagnosis of
S. pneumoniae
-caused pneumonia, and not just because of the potential for contamination of the sample by other bacteria in the mouth and/or by indigenous upper respiratory tract
S. pneumoniae
. Sputum is often difficult to collect; moreover, once medication of the patient is commenced, the number of viable
S. pneumoniae
in sputum rapidly decreases. In particular, the presence of the C-polysaccharide antigen in sputum may rapidly become difficult to detect if an antibiotic therapy is used that attacks the cell wall of the
S. pneumoniae
microorganism. When
S. pneumoniae
causes infectious otitis media, meningitis and various other aforementioned infectious disease states, sputum samples are of no aid in diagnosis.
Collection of blood cultures from patients suspected of
S. pneumoniae
infection eliminates the contamination problems that attend sputum samples. Where blood serum samples are found to contain
S. pneumoniae
, diagnosis of various diseases of which it is causative may readily be made. The drawback here is that only about 20 percent of all pneumonia patients infected by
S. pneumoniae
become bacteremic; therefore, relying solely on blood samples to diagnose
S. pneumoniae
-caused pneumonia may yield false-negative results.
Urine samples have been found to be the most reliable and convenient ones to use in detecting
S. pneumoniae
-caused pneumonia because they can be non-invasively obtained; they will not be contaminated with oral microflora; and the presence of the bacterium in urine persists, albeit at a constantly decreasing level of concentration, even after patient therapy has been initiated, so that daily monitoring of patient urine samples to assess the efficacy of a prescribed therapy may yield useful information. It should be noted that human carriers of
S. pneumoniae
who show no disease symptoms often do not have sufficient pathogen present to have
S. pneumoniae
antigens present in their urine.
A very recent article describes the successful diagnosis of meningitis caused by
S. pneumoniae
using an EIA method to test samples of cerebrospinal fluid. In the EIA, a monoclonal immunoglobulin A antiphosphoryl-choline antibody was employed to detect the C-polysaccharide antigen. See Stuertz, K., Merx, I., Eiffert, H., Schmutzhard, E., Mader, M. and Nau, R., 36
J. Clin. Microbiol
. 2346-2348. The results obtained compared favorably with those reported by Yolken, R. H., Davis, D., Winkelstein, J., Russell, H. and Sippel, J. E., 20
J. Clin. Microbiol
. 802-8
Fent Mary Kathleen
Koulchin Vladimir Andrei
Molokova Elena Valentin
Moore Norman James
BINAX, Inc.
Portner Ginny
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