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Para conocer los horarios, visitas sin turno y citas.1. Labeling. Appropriate information is critical to proper processing of test requests. Although pertinent clinical information is highly desirable, if it is not available, please provide at least the following information.
a. Patient's name
b. Source of specimen or collection site
c. Date
d. Specimen and lesion status
e. Test desired
2. Obtain specimen correctly.
a. Explain completely to the patient.
b. Use a sterile container.
c. Label correctly and send the specimen to the laboratory promptly.
d. Avoid contamination of the container.
Note: Please examine specimen collection and transportation supplies to be sure they do not include expired containers.
3. Timing of collection.
a. Sputum, urine, stool, etc. are best collected in early morning and sent to the laboratory the same day.
b. Blood
Clinical Disease Suspected | Culture Recommendation | Rationale |
---|---|---|
*Mandell Gl, Bennett JE, Dolin R, eds. Mandell, Douglas, and Bennett's Principles and Practice of Infectious Diseases. 5th ed. Philadelphia, Pa: Churchill Livingstone; 2000: 867-868. | ||
Sepsis, meningitis osteomyelitis, septic arthritis, bacterial pneumonia | Two sets of cultures − one from each of two prepared sites. Draw for the second culture after a brief time interval (30 minutes) and then begin therapy. | Assures sufficient sampling in cases of intermittent or low level bacteremia. Minimize the confusion caused by a positive culture resulting from transient bacteremia or skin contamination. |
Fever of unknown origin (eg, occult abscess, empyema, typhoid fever etc) | Two sets of cultures − one from each of two prepared sites. Draw for the second culture after a brief time interval (30 minutes). If cultures are negative after 24 to 48 hours obtain two more sets, preferably prior to an anticipated temperature rise. | The yield after four sets of cultures is minimal. |
Endocarditis: | ||
Acute | Obtain three blood culture sets within two hours, then begin therapy. | 95% to 99% of acute endocarditis patients (untreated) will yield a positive in one of the first three cultures.* |
Subacute | Obtain three blood culture sets on day one, repeat if negative after 24 hours. If still negative or if the patient had prior antibiotic therapy, repeat again. | Adequate sample volume despite low level bacteremia or previous therapy should result in a positive yield. |
Immunocompromised host aids: | ||
Septicemia, fungemia, mycobacteremia | Obtain two sets of cultures from each of two prepared sites. | Low levels of fungemia and mycobacteremia frequently encountered. |
Age | Bottle(s) | Total Blood Volume | Blood Culture Set |
---|---|---|---|
≥15 years old | 1 Aerobic (8 to 10 mL) 1 Anaerobic (8 to 10 mL) | 16 to 20 mL | 1 Set = 1 Aerobic Bottle and 1 Anaerobic Bottle |
<15 years old | 2 Pediatric (1 to 4 mL) | 2 to 8 mL | 1 Set = 2 Pediatric Bottles |
Neonates | 1 Pediatric (0.1 to 1 mL) | 0.1 to 1 mL | 1 Set = 1 Pediatric Bottle |
Anaerobic Culture. Specimens are to be collected from a prepared site using a sterile technique. Contamination with normal flora must be avoided. Some anaerobes will be killed by contact with oxygen for only a few seconds. Ideally, pus obtained by needle aspiration through intact surface, which has been aseptically prepared, is put directly into anaerobic transport media. Sampling of open lesions is enhanced by deep aspiration using a sterile plastic catheter or needle. Curettings of the base of an open lesion may also provide a good yield. If irrigation is necessary, nonbacteriostatic sterile normal saline may be used. Pulmonary samples may be obtained by transtracheal percutaneous needle aspiration or by physicians trained in this procedure. Superficial collection (ie, a swab of the lesion) is not the best specimen for anaerobic culture. If swabs must be used, two should be collected; one for culture and one for Gram stain. Swabs of the throat or genital tract are not appropriate specimens for anaerobic culture.
The following are clinical symptoms suggestive of anaerobic infection:
Upper Respiratory Tract. This section describes procedures for obtaining culture specimens from the nasopharyngeal area and the throat.
1. A nasopharyngeal culture is obtained by inserting a thin sterile swab gently through the nose to touch the pharynx; gently rotate and remove.
2. A throat culture is obtained by introducing a sterile swab into the mouth. Use a tongue blade to avoid contaminating the specimen with oral secretions. Firmly swab both tonsillar fossae, posterior pharynx, and any inflamed or ulcerated areas.
Lower Respiratory Tract: Sputum. This section discusses sputum cultures, including such alternatives as induced sputum, tracheal aspiration, and bronchial washings.
1. Rinsing the mouth with saline or water (but not mouthwash) may reduce contamination with normal oropharyngeal flora.
2. Encourage deep cough with expectoration of the sputum into a sterile specimen collection cup that is labeled with the patient's name.
3. Do not send saliva (spit) for culture.
4. When the patient is unable to cough productively, notify the physician. An alternative method may be ordered, such as:
a. Induced sputum. This is done by a respiratory therapist on the orders of the physician. Involuntary deep coughing is induced by irritation.
b. Tracheal aspiration. The trachea is gently irritated with a small lumen suction catheter, which causes deep, productive coughing. Also, the specimen may be aspirated with a syringe.
c. Bronchial washings. These are done by the physician in the operating room at the time of bronchoscopic examination. Sputum following bronchoscopy can be very productive for the recovery of mycobacteria.
5. A small amount of sputum is all that is required, but it must be sputum and not oral secretions.
6. Three sputa collected on consecutive days is recommended for the recovery of mycobacteria.
Specimens of Wound Exudate. Follow these steps for using a sterile transport swab in collecting wound exudate specimens.
1. Gently cleanse the area, using dry, sterile gauze to remove any contaminants.
2. Using a sterile bacterial culture collection system, introduce deeply enough to obtain a moist specimen; replace the swab in the container. Do not break the container.
3. Store at room temperature.
Urine for Culture. When a urine culture is ordered, follow these steps for collecting a clean-catch specimen.
1. Explain carefully to patients the mechanics of midstream collection and the importance of collecting an uncontaminated specimen. Teach them how to handle the specimen container to keep it sterile.
2. A clean-catch specimen is necessary to confirm the presence or absence of infecting organisms in urine. The specimen must be free of any contaminating matter that might be present on the genital organs; therefore, patients should be urged to follow the steps outlined below.
a. Instructions for the Female Patient.
b. Instructions for the Male Patient.
3. Cleansing agents, such as soap or detergent, must be rinsed away from the urethral area before the specimen is collected.
4. A urine specimen from a catheterized patient is obtained by using a sterile 21- to 23-gauge needle and a 3-mL syringe. Prepare an area on the distal end of the rubber catheter with an antiseptic sponge. Insert the needle at a 45° angle, pointed toward the drainage tubing. If urine is not obtained, try lifting the catheter tubing carefully. If necessary, kink the tubing three inches from the catheter and hold in place with a rubber band until urine is visible.
5. Urine for culture must be transferred to a urine transport tube that contains preservative immediately after collection.
Note: Do not collect urine specimens from a drainage bag.
Stool for Culture. When collecting stool specimens, follow these guidelines.
1. A small amount is all that is required, about the size of a walnut. If several different types of cultures are requested, submit a walnut-sized sample for each. Place the specimen in stool culture transport medium (C&S vial).
2. When stool specimens are not readily obtainable, rectal swabs are acceptable; however, it must be indicated whether the specimen is a stool or a rectal swab. Place the swab in stool culture transport medium (C&S vial).
The swab system is guaranteed sterile until the seal is broken. Directions for use:
1. Peel open and remove the swab from the package.
2. Remove the cap/swab stick from the tube.
3. Collect the appropriate specimen and put the cap/swab into the tube. Push the cap to bring the swab into contact with the transport medium.
4. Print the patient's name and the culture site on the specimen tube.
5. Place the specimen in a specimen bag and put the completed test request form in the side pouch.
6. Store it at room temperature.
7. Send specimen to the laboratory.
Normal Flora. The common practice in microbiology is to identify “significant” organisms from cultures. Significance is determined in part by the quantitation of an organism relative to other organisms present, the “pathogenicity” of isolates, and the site from which the specimen was obtained. When the organisms present are known to be part of the expected flora from a particular body site, the result reported is often “routine (site) flora”. The following list representative flora from various body sites.
Skin Flora
Respiratory Flora
The following potential pathogens may be part of the routine flora if not predominating:
Genitourinary Tract Flora