Overview of Bacterial Identification Methods and Strategies Flashcards

Question 1

Q

Differentiate microorganisms based on the ability to use acetamide as the sole source of carbon

Answer

A

Acetamide Utilization

Question 2

Q

Principle of acetamide utilization test

Answer

A

Bacteria capable of growth on this medium produce the enzyme acylamidase, which deaminates acetamide to release ammonia. The production of ammonia results in an alkaline pH, causing the medium to change color from green to royal blue

Question 3

Q

Expected results of acetamide utilization test

Answer

A

Positive: Deamination of the acetamide, resulting in a blue color
Negative: No color change

Question 4

Q

Quality control/s of acetamide utilization test

Answer

A

Positive: Pseudomonas aeruginosa—growth; blue color
Negative: Escherichia coli—no growth; green color

Question 5

Q

Differentiate organisms based on ability to use acetate as the sole source of carbon

Answer

A

Acetate Utilization

Question 6

Q

Differentiate Shigella sp. from Escherichia coli.

Answer

A

Acetate Utilization

Question 7

Q

Principle of acetate utilization test

Answer

A

Organisms capable of using sodium acetate grow on the medium, resulting in an alkaline pH, turning the indicator from green to blue

Question 8

Q

Expected results of acetate utilization test

Answer

A

Positive: Medium becomes alkalinized (blue)
Negative: No growth or growth with no indicator change to blue (green)

Question 9

Q

Quality control/s of acetate utilization test

Answer

A

Positive: Escherichia coli— growth; blue
Negative: Shigella sonnei— small amount of growth; green

Question 10

Q

This test is used for presumptive identification and differentiation of beta-hemolytic group A streptococci (Streptococcus pyogenes–susceptible) from other beta-hemolytic streptococci

Answer

A

Bacitracin Susceptibility

Question 11

Q

This test is used to distinguish staphylococci species (resistant) from micrococci (susceptible)

Answer

A

Bacitracin Susceptibility

Question 12

Q

Principle of bacitracin susceptibility test

Answer

A

The antibiotic bacitracin inhibits the synthesis of bacterial cell walls. It is placed on the agar plate and after incubation, the plate is examined for zone of inhibition

Question 13

Q

Expected result/s of bacitracin susceptibility test

Answer

A

Positive: Any zone of inhibition greater than 10 mm; susceptible
Negative: No zone of inhibition; resistant

Question 14

Q

Quality control/s of bacitracin susceptibility test

Answer

A

Positive: Streptococcus pyogenes—susceptible
Micrococcus luteus—susceptible

Negative: Streptococcus agalactiae—resistant
Staphylococcus aureus—resistant

Question 15

Q

This test is used for the presumptive identification of enterococci and organisms in the Streptococcus bovis group

Answer

A

Bile Esculin Test

Question 16

Q

This test differentiates enterococci and group D streptococci from non–group D viridans streptococci

Answer

A

Bile Esculin Test

Question 17

Q

Principle of bile esculin test

Answer

A

Gram-positive bacteria other than some streptococci and enterococci are inhibited by the bile salts in this medium. Organisms capable of growth in the presence of 4% bile and able to hydrolyze esculin to esculetin. Esculetin reacts with Fe3+ and forms a dark brown to black precipitate

Question 18

Q

Expected results of bile esculin test

Answer

A

Positive: Growth and blackening of the agar slant

Negative: Growth and no blackening of medium
No growth

Question 19

Q

Quality control/s of bile esculin test

Answer

A

Positive: Enterococcus faecalis — growth; black precipitate

Negative: Escherichia coli— growth; no color change
Streptococcus pyogenes—no growth; no color change

Question 20

Q

This test differentiates Streptococcus pneumoniae (positive–soluble) from alpha-hemolytic streptococci (negative–insoluble)

Answer

A

Bile Solubility Test

Question 21

Q

Principle of bile solubility test

Answer

A

Bile or a solution of a bile salt rapidly lyses pneumococcal colonies. Lysis depends on the presence of an intracellular autolytic enzyme, amidase. Bile salts lower the surface tension between the bacterial cell membrane and the medium, thus accelerating the organism’s natural autolytic process

Question 22

Q

Expected results of bile solubility test

Answer

A

Positive: Colony disintegrates; an imprint of the lysed colony may remain in the zone
Negative: Intact colonies

Question 23

Q

Quality control/s of bile solubility test

Answer

A

Positive: Streptococcus pneumoniae—bile soluble
Negative: Enterococcus faecalis—bile insoluble

Question 24

Q

This is a rapid test to detect the enzyme butyrate esterase, to aid identification of Moraxella (Branhamella) catarrhalis

Answer

A

Butyrate Disk

Question 25

Q

Principle of butyrate disk

Answer

A

Organisms capable of producing butyrate esterase hydrolyze bromochlorindolyl butyrate. Hydrolysis of the substrate in the presence of butyrate esterase releases indoxyl, which in the presence of oxygen spontaneously forms indigo, a blue to blue-violet color

Question 26

Q

Expected results of butyrate disk test

Answer

A

Positive: Development of a blue color during the 5-minute incubation period
Negative: No color change

Question 27

Q

Quality control/s of butyrate disk test

Answer

A

Positive: Moraxella catarrhalis— formation of blue color
Negative: Neisseria gonorrhoeae—no color change

Question 28

Q

Test used to differentiate group B streptococci (Streptococcus agalactiae– positive) from other streptococcal species

Answer

A

CAMP Test

Question 29

Q

What does CAMP Test means

Answer

A

Christie, Atkins, and Munch-Peterson (CAMP) test

Question 30

Q

Reaction of Listeria monocytogenes in CAMP Test

Answer

A

Positive CAMP reaction

Question 31

Q

Principle of CAMP test

Answer

A

Certain organisms (including group B streptococci) produce a diffusible extracellular hemolytic protein (CAMP factor) that acts synergistically with the beta-lysin of Staphylococcus aureus to cause enhanced lysis of red blood cells. The group B streptococci are streaked perpendicular to a streak of S. aureus on sheep blood agar. A positive reaction appears as an arrowhead zone of hemolysis

Question 32

Q

Expected results of CAMP test

Answer

A

Positive: Enhanced hemolysis is indicated by an arrowhead-shaped zone of beta-hemolysis at the juncture of the two organisms
Negative: No enhancement of hemolysis

Question 33

Q

Quality control/s of CAMP test

Answer

A

Positive: Streptococcus agalactiae —enhanced arrowhead hemolysis
Negative: Streptococcus pyogenes —beta-hemolysis without enhanced arrowhead formation

Question 34

Q

This test differentiates catalase-positive micrococcal and staphylococcal species from catalase-negative streptococcal species

Answer

A

Catalase Test

Question 35

Q

Principle of catalase test

Answer

A

Catalase, is capable of converting hydrogen peroxide to water and oxygen. The presence of the enzyme in a bacterial isolate is evidenced when a small inoculum introduced into hydrogen peroxide (30% for the slide test) causes rapid elaboration of oxygen bubbles

Question 36

Q

Expected results of catalase test

Answer

A

Positive: Copious bubbles are produced
Negative: No or few bubbles are produced

Question 37

Q

Quality control/s of catalase test

Answer

A

Positive: Staphylococcus aureus
Negative: Streptococcus pyogenes

Question 38

Q

This test is primarily used to isolate and purify Pseudomonas aeruginosa from contaminated specimens

Answer

A

Cetramide Agar

Question 39

Q

Principle of cetramide agar

Answer

A

The test is used to determine the ability of an organism to grow in the presence of cetrimide, a toxic substance that inhibits the growth of many bacteria by causing the release of nitrogen and phosphorous, which slows or kills the organism. P. aeruginosa is resistant to cetrimide

Question 40

Q

Expected results of cetramide agar test

Answer

A

Positive: Growth, variation in color of colonies
Negative: No growth

Question 41

Q

Quality control/s of cetramide agar test

Answer

A

Positive: Pseudomonas aeruginosa—growth and color change; yellow-green to blue-green colonies

Negative: Escherichia coli—no growth and no color change

Question 42

Q

The purpose of this test is to identify organisms capable of using sodium citrate as the sole carbon source and inorganic ammonium salts as the sole nitrogen source

Answer

A

Citrate Utilization

Question 43

Q

This test is part of a series referred to as IMViC (indole, methyl red, Voges-Proskauer, and citrate), which is used to differentiate Enterobacteriaceae from other gram-negative rods

Answer

A

Citrate Utilization

Question 44

Q

Principle of citrate utilization test

Answer

A

Bacteria that can grow on this medium produce an enzyme, citrate-permease, capable of converting citrate to pyruvate. Pyruvate can then enter the organism’s metabolic cycle for the production of energy.

Bacteria capable of growth in this medium use the citrate and convert ammonium phosphate to ammonia and ammonium hydroxide, creating an alkaline pH. The pH change turns the bromthymol blue indicator from green to blue

Question 45

Q

Expected results of citrate utilization test

Answer

A

Positive: Growth on the medium, with or without a change in the color of the indicator. Growth typically results in the bromthymol blue indicator turning from green to blue

Negative: Absence of growth

Question 46

Q

Quality control/s of citrate utilization test

Answer

A

Positive: Enterobacter aerogenes—growth, blue color
Negative: Escherichia coli—little to no growth, no color change

Question 47

Q

This test is used to differentiate Staphylococcus aureus (positive) from coagulase-negative staphylococci (negative)

Answer

A

Coagulase Test

Question 48

Q

Principle of coagulase test

Answer

A

S. aureus produces two forms of coagulase, bound and free. Bound coagulase, or “clumping factor,” is bound to the bacterial cell wall and reacts directly with fibrinogen. This results in precipitation of fibrinogen on the staphylococcal cell, causing the cells to clump when a bacterial suspension is mixed with plasma. The presence of bound coagulase correlates with free coagu- lase, an extracellular protein enzyme that causes the formation of a clot when S. aureus colonies are incubated with plasma. The clot- ting mechanism involves activation of a plasma coagulase-reacting factor (CRF), which is a modified or derived thrombin molecule, to form a coagulase-CRF complex. This complex in turn reacts with fibrinogen to produce the fibrin clot

Question 49

Q

Expected results of coagulase test (Slide test)

Answer

A

Positive: Macroscopic clumping in 10 seconds or less in coagulated plasma drop and no clumping in saline or water drop

Negative: No clumping in either drop.

Note: All negative slide tests must be confirmed using the tube test

Question 50

Q

Expected results of coagulase test (Tube test)

Answer

A

Positive: Clot of any size
Negative: No clot

Question 51

Q

Quality control/s of coagulase test

Answer

A

Positive: Staphylococcus aureus
Negative: Staphylococcus epidermidis

Question 52

Q

This test is used to differentiate decarboxylase-producing Enterobacteriaceae from other gram-negative rods

Answer

A

Decarboxylase Tests (Moeller’s Method)

Question 53

Q

Principle of Decarboxylase Tests (Moeller’s Method)

Answer

A

This test measures the enzymatic ability (decarboxylase) of an organism to decarboxylate (or hydrolyze) an amino acid to form an amine. Decarboxylation, or hydrolysis, of the amino acid results in an alkaline pH and a color change from orange to purple

Question 54

Q

Expected results of Decarboxylase Tests (Moeller’s Method)

Answer

A

Positive: Alkaline (purple) color change compared with the control tube
Negative: No color change or acid (yellow) color in test and control tube. Growth in the control tube

Question 55

Q

Quality control/s of Decarboxylase Tests (Moeller’s Method)

Answer

A

Positive:
Lysine—Klebsiella pneumoniae
Ornithine—Enterobacter aerogenes
Arginine—Enterobacter cloacae
Base—

Negative:
Lysine—Enterobacter cloacae Ornithine—Klebsiella pneumoniae
Arginine—Klebsiella pneumoniae
Base—Klebsiella pneumoniae

Question 56

Q

This test is used to distinguish Serratia sp. (positive) from Enterobacter sp., Staphylococcus aureus (positive) from other species, and Moraxella catarrhalis (positive) from Neisseria sp.

Answer

A

DNA Hydrolysis

Question 57

Q

Principle of DNA Hydrolysis Test

Answer

A

The medium is pale green because of the DNA–methyl green complex. If the organism growing on the medium hydrolyses DNA, the green color fades and the colony is surrounded by a colorless zone

Question 58

Q

Expected results of DNA Hydrolysis Test

Answer

A

Positive: COLORLESS around the test organism
Negative: Medium remains green

Question 59

Q

Quality control/s of DNA Hydrolysis Test

Answer

A

Positive: Staphylococcus aureus
Negative: Escherichia coli

Question 60

Q

This test is used for the presumptive identification and differentiation of Enterobacteriaceae

Answer

A

Esculin hydrolysis

Question 61

Q

Principle of Esculin Hydrolysis Test

Answer

A

This test is used to determine whether an organism can hydrolyze the glycoside esculin. Esculin is hydrolyzed to esculetin, which reacts with Fe3+ and forms a dark brown to black precipitate

Question 62

Q

Expected results of Esculin Hydrolysis Test

Answer

A

Positive: BLACKENED MEDIUM
Negative: No blackening

Question 63

Q

Quality control/s of Esculin Hydrolysis Test

Answer

A

Positive: Enterococcus faecalis
Negative: Escherichia coli

Question 64

Q

Media are used to differentiate organisms based on their ability to ferment carbohydrates incorporated into the basal medium

Answer

A

Fermentation media

Answer 65

A

Andrade’s Formula
Positive: Indicator change to PINK
Negative: Growth, but no change in color

Bromcresol Purple
Positive: Indicator change to YELLOW
Negative: Growth, but no change in color

Answer 66

A

Andrade’s Formula
Positive, with gas: Escherichia coli
Positive, no gas: Shigella flexneri

Bromcresol Purple
Positive, with gas: Escherichia coli
Negative, no gas: Moraxella osloensis

Answer 67

A

Flagella stain

Answer 68

A

A wet mount technique is used for staining bacterial flagella, and it is simple and useful when the number and arrangement of flagella are critical to the identification of species of motile bacteria

Answer 69

A

Peritrichous: Escherichia coli
Polar: Pseudomonas aeruginosa
Negative: Klebsiella pneumonia

Answer 70

A

Gelatin Hydrolysis Test

Answer 71

A

This test is used to determine the ability of an organism to produce extracellular proteolytic enzymes (gelatinases) that liquefy gelatin

Answer 72

A

Positive: Partial or total liquefaction at 4°C within 14 days
Negative: Complete solidification

Answer 73

A

Positive: Bacillus subtilis
Negative: Escherichia coli

Answer 74

A

Growth at 42 C

Answer 75

A

The test is used to determine the ability of an organism to grow at 42°C. Several Pseudomonas species have been isolated in the clinical laboratory that are capable of growth at elevated temperatures

Answer 76

A

Positive: Good growth at both 35°and 42°C
Negative: No growth at 42°C but good growth at 35°C

Answer 77

A

Positive: Pseudomonas aeruginosa
Negative: Pseudomonas fluorescens

Answer 78

A

Hippurate Hydrolysis

Answer 79

A

The end products of hydrolysis of hippuric acid by hippuricase include glycine and benzoic acid. Glycine is deaminated by the oxidizing agent ninhydrin, which is reduced during the process. The end products of the ninhydrin oxidation react to form a purple-colored product. The test medium must contain only hippurate because ninhydrin might react with any free amino acids present in growth media or other broths

Answer 80

A

Positive: Deep purple color
Negative: Colorless or slightly yellow pink color

Answer 81

A

Positive: Streptococcus agalactiae
Negative: Streptococcus pyogenes

Answer 82

A

Indole Production Test

Answer 83

A

Indole Production Test

Answer 84

A

The indole test detects tryptophanase production and determines the ability of a
microorganism to produce indole from the degradation of the amino acid tryptophan. The test is used to determine an organism’s ability to hydrolyze tryptophan to form the
compound indole

Answer 85

A

Positive: PINK- TO WINE-COLORED RING
Negative: No color change

Answer 86

A

A. KOVAC’S METHOD
- Positive: Escherichia coli
- Negative: Klebsiella pneumoniae
B. EHRLICH’S METHOD
- Positive: Haemophilus influenzae
- Negative: Haemophilus parainfluenzae C. EHRLICH’S METHOD (ANAEROBIC)
- Positive: Porphyromonas asaccharolytica
- Negative: Bacteroides fragilis

Answer 87

A

Leucine Aminopeptidase (LAP) Test

Answer 88

A

The LAP disk is a rapid test for the detection of the enzyme leucine aminopeptidase. Leucinebeta- naphthylamide– impregnated disks serve as a substrate for the detection of leucine aminopeptidase. After hydrolysis of the substrate by the enzyme, the resulting beta- naphthylamine produces a red color upon addition of cinnamaldehyde reagent

Answer 89

A

Positive: Development of a red color within 1 minute
Negative: No color change or development of a slight yellow color

Answer 90

A

Positive: Enterococcus faecalis
Negative: Aerococcus viridans

Answer 91

A

Litmus Milk Medium

Answer 92

A

Fermentation of lactose is demonstrated when the litmus turns pink as a result of acid production. If sufficient acid is produced, casein in the milk is coagulated, solidifying the milk. With some organisms, the curd shrinks, and whey is formed at the surface. Some bacteria hydrolyze casein, causing the milk to become straw colored and resemble turbid serum. Additionally, some organisms reduce litmus, in which case the medium becomes colorless in the bottom of the tube

Answer 93

A

Fermentation: Clostridium perfringens
Acid: Lactobacillus acidophilus
Peptonization: Pseudomonas aeruginosa

Answer 94

A

Lysine Iron Agar (LIA)

Answer 95

A

When glucose is fermented, the butt of the medium becomes acidic (yellow). If the organism produces lysine decarboxylase, cadaverine is formed. Cadaverine neutralizes the organic acids formed by glucose fermentation, and the butt of the medium reverts to the alkaline state (purple). If the decarboxylase is not produced, the butt remains acidic (yellow). If oxidative deamination of lysine occurs, a compound is formed that, in the presence of ferric ammonium citrate and a coenzyme, flavin mononucleotide, forms a burgundy color on the slant. If deamination does not occur, the LIA slant remains purple.

Answer 96

A

Methyl Red / Voges-Proskauer (MRVP) Test

Answer 97

A

This test is used to determine the ability of an organism to produce and maintain stable acid end products from glucose fermentation, to overcome the buffering capacity of the system, and to determine the ability of some organisms to produce neutral end products (e.g., 2,3-butanediol or acetoin) from glucose fermentation

Answer 98

A

Positive: Red color, indicative of acetoin production
Negative: Yellow color

Answer 99

A

MR positive/VP negative: Escherichia coli
MR negative:/VP positive: Enterobacter aerogenes

Answer 100

A

Microdase Test (Modified Oxidase)

Answer 101

A

The microdase test is a rapid method to differentiate Staphylococcus from Micrococcus spp. by detection of the enzyme oxidase. In the presence of atmospheric oxygen, the oxidase enzyme reacts with the oxidase reagent and cytochrome C to form the colored compound, indophenol

Answer 102

A

Positive: Development of BLUE TO PURPLE-BLUE COLOR
Negative: NO COLOR CHANGE

Answer 103

A

Positive: Micrococcus luteus
Negative: Staphylococcus aureus

Answer 104

A

Motility Testing

Answer 105

A

The inoculum is stabbed into the center of a semisolid agar deep. Bacterial motility is evident by a diffuse zone of growth extending out from the line of inoculation. Some organisms grow throughout the entire medium, whereas others show small areas or nodules that grow out from the line of inoculation

Answer 106

A

Positive: Spread out from the site of inoculation
Negative: Remain at the site of inoculation

Answer 107

A

Positive: Escherichia coli
Negative: Staphylococcus aureus

Answer 108

A

De Man, Rogosa and Sharpe (MRS) Broth

Answer 109

A

The MRS broth contains sources of carbon, nitrogen, and vitamins to support the growth of lactobacilli and other organisms. It is a selective medium that uses sodium acetate and ammonium citrate to prevent overgrowth by contaminating organisms. Growth is considered a positive result

Answer 110

A

Positive: Leuconostoc sp.: Growth, gas production indicated by a bubble in the Durham tube
Positive: Lactobacillus spp.: Growth, no gas production
Negative: No growth

Answer 111

A

Positive: Lactobacillus lactis
Negative: Escherichia coli

Answer 112

A

4-Methylumbelliferyl-β-D-Glucuronide (MUG) Test

Answer 113

A

E. coli and other Enterobacteriaceae produce the enzyme β-d-glucuronidase, which hydrolyzes β-d-glucopyranosid-uronic derivatives to aglycons and d-glucuronic acid. The substrate 4-methylumbelliferyl-β-d-glucuronide is impregnated into the disk and is hydrolyzed by the enzyme to yield the 4-methylumbelliferyl moiety, which fluoresces blue under long wavelength ultraviolet light. However, verotoxin producing strains of E. coli do not produce MUG, and a negative test result may indicate the presence of a clinically important strain

Answer 114

A

Positive: Electric blue fluorescence
Negative: Lack of fluorescence

Answer 115

A

Positive: Escherichia coli
Negative: Klebsiella pneumoniae

Answer 116

A

Nitrate Reduction Test

Answer 117

A

Positive: RED
Negative: No color change

Answer 118

A

Positive: NO3+, no gas: Escherichia coli
Positive: NO3+, gas: Pseudomonas aeruginosa
Negative: Acinetobacter baumannii

Answer 119

A

Nitrite Reduction Test

Answer 120

A

Microorganisms capable of reducing nitrite to nitrogen do not turn color and do produce gas in the nitrate reduction test

Answer 121

A

Positive: No color change to red 2 minutes; gas production in Durham tube
Negative: Broth becomes red; no gas production is observed

Answer 122

A

Positive: Proteus mirabilis
Negative: Acinetobacter baumannii

Answer 123

A

O-NITROPHENYL-Β-D-GALACTOPYRANOSIDE (ONPG) TEST

Answer 124

A

O-NITROPHENYL-Β-D-GALACTOPYRANOSIDE (ONPG) TEST

Answer 125

A

Lactose fermenters must be able to transport the carbohydrate (β-galactoside permease) and hydrolyze (β-galactosidase) the lactose to glucose and galactose. Organisms unable to produce β-galactosidase may become genetically altered through a variety of mechanisms and be identified as late-lactose fermenters. ONPG enters the cells of organisms that do not produce the permease but are capable of hydrolyzing the ONPG to galactose and a yellow compound, o-nitrophenol, indicating the presence of β-galactosidase

Answer 126

A

Positive: YELLOW (presence of β-galactosidase)
Negative: Colorless

Answer 127

A

Positive: Shigella sonnei
Negative: Salmonella typhimurium

Answer 128

A

Optochin (P disk) Susceptibility Test

Answer 129

A

Optochin is an antibiotic that interferes with the ATPase and production of adenosine triphosphate (ATP) in microorganisms. The Optochin impregnated disk (TaxoP) is placed on a lawn of organism on a sheep blood agar plate, allowing the antibiotic to diffuse into the medium. The antibiotic inhibits the growth of a susceptible organism, creating a clearing, or zone of inhibition, around the disk. A zone of 14 to 16 mm is considered susceptible and presumptive identification for Streptococcus pneumoniae

Answer 130

A

Positive: ZOI ≥ 14 mm in diameter, with 6-mm disk
Negative: No zone of inhibition

Answer 131

A

Positive: Streptococcus pneumoniae
Negative: Streptococcus pyogenes

Answer 132

A

Oxidase Test (Kovac’s Method)

Answer 133

A

Oxidase Test (Kovac’s Method)

Answer 134

A

To determine the presence of bacterial cytochrome oxidase using the oxidation of the substrate tetramethyl-p-phenylenediamine dihydrochloride to indophenol, a dark purple colored end product. A positive test (presence of oxidase) is indicated by the development of a dark purple color. No color development indicates a negative test and the absence of the enzyme

Answer 135

A

Positive: Development of a dark purple color within 10 seconds
Negative: Absence of color

Answer 136

A

Positive: Pseudomonas aeruginosa
Negative: Escherichia coli

Answer 137

A

Oxidation/Fermentation (of) Medium (CDC Method)

Answer 138

A

Positive: Acid production (A) indicated by the color indicator changing to yellow
Weak-positive (Aw): Weak acid formation
Negative: Red or alkaline (K) color in the deep
No change (NC) or neutral (N)

Answer 139

A

Fermenter (Glucose): Escherichia coli
Oxidizer (Glucose): Pseudomonas aeruginosa

Answer 140

A

Phenylalanine Deaminase Agar

Answer 141

A

Phenylalanine Deaminase Agar

Answer 142

A

Microorganisms that produce phenylalanine deaminase remove the amine (NH2) from phenylalanine. The reaction results in the production of ammonia (NH3) and phenylpyruvic acid. The phenylpyruvic acid is detected by adding a few drops of 10% ferric chloride; a green colored complex is formed between these two compounds

Answer 143

A

Positive: GREEN COLOR on slant
Negative: Slant remains original color

Answer 144

A

Positive: Proteus mirabilis
Negative: Escherichia coli

Answer 145

A

L-Pyrrolidonyl Arylamidase (PYR) Test

Answer 146

A

The enzyme L-pyrrolidonyl arylamidase hydrolyzes the L-pyrrolidonyl-β-naphthylamide substrate to produce a β-naphthylamine. The β-naphthylamine can be detected in the presence of N,N-methylaminocinnamaldehyde reagent by the production of a bright red precipitate

Answer 147

A

Positive: Bright red color within 5 minutes
Negative: No color change or an orange color

Answer 148

A

Positive: Enterococcus faecalis, Streptococcus pyogenes
Negative: Streptococcus agalactiae

Answer 149

A

Pyruvate Broth

Answer 150

A

Pyruvate Broth

Answer 151

A

Pyruvate broth is a carbohydrate-free, nutrient limited medium. Pyruvic acid is added to the broth to determine whether the microorganism is able to use pyruvate, resulting in the formation of metabolic acids. Bromthymol blue indicator changes from blue to yellow in the presence of acid as a result of the decrease in pH

Answer 152

A

Positive: Indicator changes from green to yellow
Negative: No color change

Answer 153

A

Positive: Enterococcus faecalis
Negative: Streptococcus bovis

Answer 154

A

Salt Tolerance Test

Answer 155

A

Salt Tolerance Test

Answer 156

A

The salt tolerance test is a selective and differential medium. Enterococci are resistant to high salt concentration. A heart infusion broth containing 6.5% NaCl is used as the test medium. This broth also contains a small amount of glucose and bromcresol purple as the indicator for acid production

Answer 157

A

Positive: Visible turbidity in the broth, with or without a color change from purple to yellow
Negative: No turbidity and no color change

Answer 158

A

Positive: Enterococcus faecalis
Negative: Streptococcus bovis

Answer 159

A

Spot Indole Test

Answer 160

A

Tryptophanase breaks down tryptophan to release indole, which is detected by its ability to combine with certain aldehydes to form a colored compound. For indole-positive bacteria, the blue-green compound formed by the reaction of indole with cinnamaldehyde is easily visualized. The absence of enzyme results in no color production (indole negative

Answer 161

A

Positive: Development of a blue color within 20 seconds
Negative: No color development or slightly pink color

Answer 162

A

Positive: Escherichia coli
Negative: Klebsiella pneumoniae

Answer 163

A

Triple Sugar Iron (TSI) Agar

Answer 164

A

Triple sugar iron agar contains three sugars (lactose, sucrose, and glucose), ferrous sulfate, and a pH indicator.

COMPOSITION: 10 parts Lactose, 10 parts sucrose, 1 part glucose and peptone

Phenol Red: pH indicator

Ferrous Ammonium Sulfate: H2S Indicator

CO2 and hydrogen gas (H2): presence of bubbles or cracks or by separation of the agar

Answer 165

A

Acid reaction (A): yellow color
Alkaline reaction (K): red color
Hydrogen sulfide production (H2S): black color or precipitate
Gas production (G): bubbles, cracks, or media displacement

Answer 166

A

Alkaline slant/ Alkaline butt (K/K): glucose, lactose, and sucrose nonutilizer

Alkaline slant/Acid butt (K/A): glucose fermentation only

Acid slant/Acid butt (A/A): glucose, sucrose, and/or lactose fermenter

Black Precipitate: production of ferrous sulfide and H2S gas (H2S+)

Bubbles or cracks: gas production

Answer 167

A

A/A gas production: Escherichia coli

K/A, +/− gas production, H2S+: Salmonella typhimurium

K/K: Pseudomonas aeruginosa

K/A, H2S+: Proteus mirabilis

K/A: Shigella flexneri

Answer 168

A

Urea Test (Christensen’s Method)

Answer 169

A

Urea is the product of decarboxylation of amino acids. Hydrolysis of urea produces ammonia and CO2. The formation of ammonia alkalinizes the medium, and the pH shift is detected by the color change of phenol red from light orange at pH 6.8 to magenta (pink) at pH 8.1. Rapid urease-positive organisms turn the entire medium pink within 24 hours. Weakly positive organisms may take several days, and negative organisms produce no color change or yellow as a result of acid production

Answer 170

A

Positive: Change in color of slant from light orange to magenta
Negative: No color change

Answer 171

A

Positive: Proteus vulgaris
Weak positive: Klebsiella pneumonia
Negative: Escherichia coli

Answer 172

A

X and V Factor Test

Answer 173

A

Members of the genus Haemophilus require accessory growth factors in vitro. Some Haemophilus spp. require X factor (hemin) alone, V factor (nicotinamide adenine dinucleotide [NAD]) alone, or a combination of the two

The organisms will grow only around the disk that provides the appropriate factor for growth of the organism

Answer 174

A

Positive:
Growth around the XV disk: requirement for both factors

Growth around the V disk, no growth around the X disk, and light growth around the XV disk shows a V factor requirement

Negative: Growth over the entire surface of the agar indicates no requirement for either X or V factor

Answer 175

A

Haemophilus influenza: halo of growth around the XV disk, no growth on the rest of the agar surface

Haemophilus parainfluenzae: halo of growth around the XV and V disks

Haemophilus ducreyi: halo of growth around the XV and X disks

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