Information about Gram Stain
Gram-positive anthrax bacteria (purple rods) in cerebrospinal fluid sample. If present, a Gram-negative bacterial species would appear pink. (The other cells are white blood cells).
Gram staining (or Gram's method) is an empirical method of differentiating bacterial species into two large groups (Gram-positive and Gram-negative) based on the chemical and physical properties of their cell walls.[1]
The method is named after its inventor, the Danish scientist Hans Christian Gram (1853–1938), who developed the technique in 1884 to discriminate between pneumococci and Klebsiella pneumoniae bacteria.[2]
Uses
Research
Gram staining is a common procedure in the traditional bacteriological laboratory.[3] The technique is used as a tool for the differentiation of Gram-positive and Gram-negative bacteria, as a first step to determine the identity of a particular bacterial sample.[4]The Gram stain is not an infallible tool for diagnosis, identification, or phylogeny, however. It is of extremely limited use in environmental miwow, and has been largely superseded by molecular techniques even in the medical microbiology lab. Given that some organisms are gram-variable (i.e. they may stain either negative or positive), and that some organisms are not susceptible to either stain used by the Gram technique, its true utility to researchers should be considered limited and specific. In a modern environmental or molecular microbiology lab, most identification is done using genetic sequences and other molecular techniques, which are far more specific and information-rich than differential staining.
Medical
Gram stains are performed on body fluid or biopsy when infection is suspected. It yields results much more quickly than culture, and is especially important when infection would make an important difference in the patient's treatment and prognosis; examples are cerebrospinal fluid for meningitis and synovial fluid for septic arthritis.[4][5]As a general rule of thumb (which has exceptions), Gram-negative bacteria are more pathogenic due to their outer membrane structure. The presence of a capsule will often increase the virulence of a pathogen. Additionally, Gram-negative bacteria have lipopolysaccharide in their outer membrane, an endotoxin which increases the severity of inflammation. This inflammation may be so severe that septic shock may occur. Gram-positive infections are generally less severe because the human body does not contain peptidoglycan; in fact, humans produce an enzyme (lysozyme) that attacks the open peptidoglycan layer of Gram-positive bacteria. Gram-positive bacteria are also frequently much more susceptible to beta-lactam antibiotics, such as penicillin.
Exceptions to the rule include branching and filamentous Gram-positive bacteria such as Mycobacterium tuberculosis and other agents of tuberculosis, or Nocardia species, the agents of nocardiosis and some types of actinomycetoma. These organisms present unique problems in diagnosis and treatment, and special stains such as the Ziehl-Neelsen stain and the Kinyoun stain are used in their laboratory workup.
Staining mechanism
Gram-positive bacteria have a thick mesh-like cell wall made of peptidoglycan (90% of cell wall), which stain purple and Gram-negative bacteria have a thinner layer (10% of cell wall), which stain pink. Gram-negative bacteria also have an additional outer membrane which contains lipids, and is separated from the cell wall by the periplasmic space. There are four basic steps of the Gram stain, which include applying a primary stain (crystal violet) to a heat-fixed smear of a bacterial culture, followed by the addition of a mordant (Gram's iodine), rapid decolorization with alcohol or acetone, and counterstaining with safranin or basic fuchsin.Crystal violet (CV) dissociates in aqueous solutions into CV+ and chloride (Cl–) ions. These ions penetrate through the cell wall and cell membrane of both Gram-positive and Gram-negative cells. The CV+ ion interacts with negatively charged components of bacterial cells and stains the cells purple. Iodine (I– or I3–) interacts with CV+ and forms large complexes of crystal violet and iodine (CV–I) within the inner and outer layers of the cell. When a decolorizer such as alcohol or acetone is added, it interacts with the lipids of the cell membrane. A Gram-negative cell will lose its outer membrane and the peptidoglycan layer is left exposed. The CV–I complexes are washed from the Gram-negative cell along with the outer membrane. In contrast, a Gram-positive cell becomes dehydrated from an ethanol treatment. The large CV–I complexes become trapped within the Gram-positive cell due to the multilayered nature of its peptidoglycan. The decolorization step is critical and must be timed correctly; the crystal violet stain will be removed from both Gram-positive and negative cells if the decolorizing agent is left on too long (a matter of seconds).
After decolorization, the Gram-positive cell remains purple and the Gram-negative cell loses its purple color. Counterstain, which is usually positively-charged safranin or basic fuchsin, is applied last to give decolorized Gram-negative bacteria a pink or red color.[6][7]
Some bacteria, after staining with the Gram stain, yield a Gram-variable pattern: a mix of pink and purple cells are seen. The genera Actinomyces, Arthobacter, Corynebacterium, Mycobacterium, and Propionibacterium have cell walls particularly sensitive to breakage during cell division, resulting in Gram-negative staining of these Gram-positive cells. In cultures of Bacillus, Butyrivibrio, and Clostridium a decrease in peptidoglycan thickness during growth coincides with an increase in the number of cells that stain Gram-negative[8] In addition, in all bacteria stained using the Gram stain, the age of the culture may influence the results of the stain.
Gram staining protocol
- Make a slide of tissue or body fluid that is to be stained. Heat the slide for few seconds until it becomes hot to the touch so that bacteria are firmly mounted to the slide.
- Add the primary stain crystal violet and incubate 1 minute. This step colors all cells violet.
- Add Gram's iodine, for 30 seconds. It is not a stain; it is a mordant. It doesn't give color directly to the bacteria but it fixes the crystal violet to the bacterial cell wall. All cells remain violet.
- Wash with ethanol and acetone, the Decolorizer. If the bacteria is Gram-positive it will retain the primary stain. If it is Gram-negative it will lose the primary stain and appear colorless.
- Add the secondary stain, safranin, and incubate 1 min, then wash with water for a maximum of 5 seconds. If the bacteria is Gram-positive then the cell will retain the primary stain, will not take the secondary stain, and will appear black-violet. If the bacteria is Gram-negative then the cell will lose the primary stain, take secondary stain, and will appear red-pink.
Gram Stain is 2 g of 90% crystal violet dissolved in 20 ml of 95% ethyl alcohol.
Gram's iodine is 1 g of iodine, 2 g of potassium iodide, dissolved in 300 ml of distilled water.
Decolorizer is 50% ethyl alcohol, 50% acetone.
In addition it is now common to use basic fuchsin instead of safranin.
See also
References
1. ^ Bergey, David H.; John G. Holt; Noel R. Krieg; Peter H.A. Sneath (1994). Bergey's Manual of Determinative Bacteriology, 9th ed., Lippincott Williams & Wilkins. ISBN 0-683-00603-7.
2. ^ Gram, HC (1884). "Über die isolierte Färbung der Schizomyceten in Schnitt- und Trockenpräparaten". Fortschritte der Medizin 2: 185-89.
3. ^ Ryan KJ; Ray CG (editors) (2004). Sherris Medical Microbiology, 4th ed., McGraw Hill, 232 – 3. ISBN 0838585299.
4. ^ Madigan, MT; Martinko J; Parker J (2004). Brock Biology of Microorganisms, 10th Edition, Lippincott Williams & Wilkins. ISBN 0-13-066271-2.
5. ^ Søgaard M, Nørgaard M, Schønheyder H (2007). "First notification of positive blood cultures: high accuracy of the Gram stain report (Epub ahead of publication)". J Clin Microbiol. PMID 17301283.
6. ^ Beveridge, T.J.; Davies, J.A.. "Cellular responses of Bacillus subtilis and Escherichia coli to the Gram stain" (PDF). J. Bacteriol. 156 (2): 846-858. PMID 6195148. Retrieved on 2007-02-17.
7. ^ Davies, J.A.; G.K. Anderson, T.J. Beveridge, H.C. Clark. "Chemical mechanism of the Gram stain and synthesis of a new electron-opaque marker for electron microscopy which replaces the iodine mordant of the stain" (PDF). J. Bacteriol. 156 (2): 837-845. PMID 6195147. Retrieved on 2007-02-17.
8. ^ Beveridge, T.J.. "Mechanism of gram variability in select bacteria" (PDF). J. Bacteriol. 172 (3): 1609-1620. PMID 1689718. Retrieved on 2007-02-17.
2. ^ Gram, HC (1884). "Über die isolierte Färbung der Schizomyceten in Schnitt- und Trockenpräparaten". Fortschritte der Medizin 2: 185-89.
3. ^ Ryan KJ; Ray CG (editors) (2004). Sherris Medical Microbiology, 4th ed., McGraw Hill, 232 – 3. ISBN 0838585299.
4. ^ Madigan, MT; Martinko J; Parker J (2004). Brock Biology of Microorganisms, 10th Edition, Lippincott Williams & Wilkins. ISBN 0-13-066271-2.
5. ^ Søgaard M, Nørgaard M, Schønheyder H (2007). "First notification of positive blood cultures: high accuracy of the Gram stain report (Epub ahead of publication)". J Clin Microbiol. PMID 17301283.
6. ^ Beveridge, T.J.; Davies, J.A.. "Cellular responses of Bacillus subtilis and Escherichia coli to the Gram stain" (PDF). J. Bacteriol. 156 (2): 846-858. PMID 6195148. Retrieved on 2007-02-17.
7. ^ Davies, J.A.; G.K. Anderson, T.J. Beveridge, H.C. Clark. "Chemical mechanism of the Gram stain and synthesis of a new electron-opaque marker for electron microscopy which replaces the iodine mordant of the stain" (PDF). J. Bacteriol. 156 (2): 837-845. PMID 6195147. Retrieved on 2007-02-17.
8. ^ Beveridge, T.J.. "Mechanism of gram variability in select bacteria" (PDF). J. Bacteriol. 172 (3): 1609-1620. PMID 1689718. Retrieved on 2007-02-17.
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In philosophy generally, empiricism is a theory of knowledge emphasizing the role of experience, especially sensory perception, in the formation of ideas, while discounting the notion of innate ideas.
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Bacteria
Phyla
Actinobacteria
Aquificae
Chlamydiae
Bacteroidetes/Chlorobi
Chloroflexi
Chrysiogenetes
Cyanobacteria
Deferribacteres
Deinococcus-Thermus
Dictyoglomi
Fibrobacteres/Acidobacteria
Firmicutes
Fusobacteria
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Phyla
Actinobacteria
Aquificae
Chlamydiae
Bacteroidetes/Chlorobi
Chloroflexi
Chrysiogenetes
Cyanobacteria
Deferribacteres
Deinococcus-Thermus
Dictyoglomi
Fibrobacteres/Acidobacteria
Firmicutes
Fusobacteria
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Gram-positive bacteria are those that retain a crystal violet dye during the Gram stain process.[1] Gram-positive bacteria appear blue or violet under a microscope, while Gram-negative bacteria appear red or pink.
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Gram-negative bacteria are those that do not retain crystal violet dye in the Gram staining protocol.[1] Gram-positive bacteria will retain the dark blue dye after an alcohol wash.
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cell wall is a fairly rigid layer surrounding a cell, located external to the cell membrane, which provides the cell with structural support, protection, and acts as a filtering mechanism. The cell wall also prevents over-expansion when water enters the cell.
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Motto
none
(Royal motto: Guds hjælp, Folkets kærlighed, Danmarks styrke
"The Help of God, the Love of the People, the Strength of Denmark" )
Anthem
Der er et yndigt land (national)
Kong Christian
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none
(Royal motto: Guds hjælp, Folkets kærlighed, Danmarks styrke
"The Help of God, the Love of the People, the Strength of Denmark" )
Anthem
Der er et yndigt land (national)
Kong Christian
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Hans Christian Joachim Gram (September 13, 1853 - November 14, 1938) was a Danish bacteriologist. He was the son of Frederik Terkel Julius Gram, a professor of jurisprudence, and Louise Christiane Roulund.
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18th century - 19th century - 20th century
1850s 1860s 1870s - 1880s - 1890s 1900s 1910s
1881 1882 1883 - 1884 - 1885 1886 1887
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Subjects: Archaeology - Architecture -
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1850s 1860s 1870s - 1880s - 1890s 1900s 1910s
1881 1882 1883 - 1884 - 1885 1886 1887
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S. pneumoniae
Binomial name
Streptococcus pneumoniae
(Klein 1884)
Chester 1901
Streptococcus pneumoniae, or pneumococcus
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Binomial name
Streptococcus pneumoniae
(Klein 1884)
Chester 1901
Streptococcus pneumoniae, or pneumococcus
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Klebsiella pneumoniae
Classification & external resources
ICD-10 B 96.1 , G 00.8 , J 15.0 , P 23.6
ICD-9 041.3 , 320.82 , 482.0
DiseasesDB 7181
eMedicine med/1237
MeSH C01.252.400.310.
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Classification & external resources
ICD-10 B 96.1 , G 00.8 , J 15.0 , P 23.6
ICD-9 041.3 , 320.82 , 482.0
DiseasesDB 7181
eMedicine med/1237
MeSH C01.252.400.310.
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Microbiology is the study of microorganisms, which are unicellular or cell-cluster microscopic organisms.[1] This includes eukaryotes such as fungi and protists, and prokaryotes such as bacteria and certain algae.
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laboratory (informally, lab) is a facility that provides controlled conditions in which scientific research, experiments, and measurement may be performed. The title of laboratory
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Bodily fluids listed below are found in the bodies of men and/or women. Some may be found in animals as well. They include fluids that are excreted or secreted from the body as well as fluids that normally are not.
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A biopsy (in Greek: bios = life and opsy = look/appearance) is a medical test involving the removal of cells or tissues for examination. The tissue is generally examined under a microscope by a pathologist, and can also be analyzed chemically (for example, using
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An infection is the detrimental colonization of a host organism by a foreign species. In an infection, the infecting organism seeks to utilize the host's resources to multiply (usually at the expense of the host).
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A microbiological culture, or microbial culture, is a method of growing a microbial organism to determine what it is, its abundance in the sample being tested, or both. It is one of the primary diagnostic methods of microbiology.
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Cerebrospinal fluid (CSF), Liquor cerebrospinalis, is a clear bodily fluid that occupies the subarachnoid space and the ventricular system around and inside the brain.
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Meningitis
Classification & external resources
Meninges of the central nervous system: dura mater, arachnoid, and pia mater.
ICD-10 G 00. -G 03.
ICD-9 320 - 322
DiseasesDB 22543
MedlinePlus 000680
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Classification & external resources
Meninges of the central nervous system: dura mater, arachnoid, and pia mater.
ICD-10 G 00. -G 03.
ICD-9 320 - 322
DiseasesDB 22543
MedlinePlus 000680
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Synovial fluid is a thick, stringy fluid found in the cavities of synovial joints. With its egg-like consistency (synovial comes from Latin for "egg"), synovial fluid reduces friction between the articular cartilage and other tissues in joints to lubricate and cushion them
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Septic arthritis
Classification & external resources
ICD-10 M00-M03
ICD-9 711.0
eMedicine med/3394
Septic arthritis is the invasion of the joint space by an infectious agent which produces arthritis.
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Classification & external resources
ICD-10 M00-M03
ICD-9 711.0
eMedicine med/3394
Septic arthritis is the invasion of the joint space by an infectious agent which produces arthritis.
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A pathogen or infectious agent is a biological agent that causes disease or illness to its host.[1] The term is most often used for agents that disrupt the normal physiology of a multicellular animal or plant.
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The word capsule, or encapsulation, may refer to:
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- Capsule (anatomy), a cover or envelope partly or wholly surrounding a structure.
- Capsule (fruit), a type of dry fruit like the poppy, iris or foxglove.
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A pathogen or infectious agent is a biological agent that causes disease or illness to its host.[1] The term is most often used for agents that disrupt the normal physiology of a multicellular animal or plant.
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Lipopolysaccharide (LPS) is a large molecule consisting of a lipid and a polysaccharide (carbohydrate) joined by a covalent bond.
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Functions
LPS is a major component of the outer membrane of Gram-negative bacteria, contributing greatly to the structural integrity of..... Click the link for more information.
Endotoxins are potentially toxic, natural compounds found inside pathogens such as bacteria. Classically, an "endotoxin" is a toxin, which unlike an "exotoxin", is not secreted in soluble form by live bacteria, but is a structural component in the bacteria which is released
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Inflammation (Latin, inflammatio, to set on fire) is the complex biological response of vascular tissues to harmful stimuli, such as pathogens, damaged cells, or irritants.
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Septic shock
Classification & external resources
ICD-10 A41.9
ICD-9 785.52
Septic shock is a serious medical condition caused by decreased tissue perfusion and oxygen delivery as a result of infection and sepsis.
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Classification & external resources
ICD-10 A41.9
ICD-9 785.52
Septic shock is a serious medical condition caused by decreased tissue perfusion and oxygen delivery as a result of infection and sepsis.
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Peptidoglycan, also known as murein, is a polymer consisting of sugars and amino acids that forms a mesh-like layer outside the plasma membrane of eubacteria. The sugar component consists of alternating residues of β-(1,4) linked N-acetylglucosamine and N-acetylmuramic
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Enzymes are proteins that catalyze (i.e. accelerate) chemical reactions.[1] In enzymatic reactions, the molecules at the beginning of the process are called substrates, and the enzyme converts them into different molecules, the products.
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Lysozyme is a 14.4 kilodalton enzyme (EC 3.2.1.17 ) that damages bacterial cell walls by catalyzing hydrolysis of 1,4-beta-linkages between N-acetylmuramic acid and N-acetyl-D-glucosamine residues in a peptidoglycan and between N-acetyl-D-glucosamine residues in chitodextrins.
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