Chapter 18

Question 1

A) What is naturally acquired immunity? [Figure 18.2]

Answer 1

Immunity that occurs through natural events.Immunity in which your body aquires it’s own imunity, or through breast milk of mother

Question 2

B) What is artificially acquired immunity? [Figure 18.2]

Answer 2

I.e. vaccinations

Question 3

C) What is active immunity? How does it develop?’

Answer 3

Active is developed by being exposed to a illness and you body makes memory cells.

Question 4

D) How does passive immunity occur? Does it have memory?

Answer 4

When you receive antibodies, your body doesn’t have to make some antigens. during pregnancy and breastfeeding.

Question 5

1) What is a antiserum?

Answer 5

serum ( fluid portion of blood) that contains protective anitbodies

Question 6

2) What do antitoxins protect against?

Answer 6

They neutralize toxins

Question 7

E) What is hyperimmune globulin used for? How is it prepared?

Answer 7

prepared from sera of donors with high amounts of antibodies for certain disease agents. these are given during incubation period it can prevent infection. There is one for tetanus, rabis, and hep b.

Question 8

F) What is immune globulin used for? How is it prepared?

Answer 8

IgG from many plasma donors. This has many different kinds of antibodies. These are used for the immunosupressed or those not vaccinated

Question 9

A) What is a vaccine? How do they work?

Answer 9

Can either be live, or dead virus/ bacteria. It is introduced to body so the body can get memory t cells without getting infection. Prepararation of a pathogen/ produces used to induce active immunity

Question 10

C) What are the differences between attenuated and inactivated vaccines?

Answer 10

C. Attenuated are “live strains”. that are in weakened form and generally do not cause disease. They can be given orally, nasal, or as shot. They are used to mimic the disease in how it enters body and as it multiplies making body make immune response. Single dose is enough for long lasting immunity… because they can multiply and are in body longer. And can spread to other immunizing them
, the inactivated are “dead strains”
unable to replicate. cannot cause infection. Requires multiple doses for long lasting immunity. have 3 types innactivated whole agent, toxoids, and subunit vaccines, recombinant, VLP. polysacharide, and conjugate vaccines.

Question 11

1) How are inactivated whole agent vaccines made, what do they treat?

Answer 11

ie influenza rabis, and polio.

Made by chemically treating, mainly with formalin that doesn’t alter eptitopes, but cannot reproduce

Question 12

2) What are toxoids, what do they treat?

Answer 12

treat toxins to destroy the toxic part of molecules, while retaining the antigentic epitopes.
ie diptheria, tetanus

Question 13

3) How are subunit vaccines made and what are the advantages of using them.

Answer 13

contain key protien antigens. they can take out ones that elicit unwanted side effects

Question 14

4) What are recombinant vaccines? Give an example.

Answer 14

genetically engineered microorganisms. ie take yeast and engineer so produce part of a viral protien coat.ie. hept b

Question 15

5) What are VLP vaccines? Give an example.

Answer 15

empty capsids which produce segments of capsid viral protien coats that self assemble. Ie HPV vaccine

Question 16

6) What are polysaccharide vaccines? Why are they ineffective in children?

Answer 16

because they are t independant antigens that illicit a poor response in kids. ie pneumococcus vaccines

Question 17

7) What are conjugate vaccines? Give an example.

used for? How do they work? [Figure 18.3]

Answer 17

ie. menningitis ( Haemeophilus influenzae).

polysacharides linked to protiens. this converts poysacharides to t dependent antigens..

Question 18

8) What are adjuvants? Why are they necessary? Why are some unsuitable for humans?

Answer 18

substances that enhance immune response to an antigen. these are important cause many lack vaccines like toqoids do not elicit danger signals. believed to provide danger signals to dendrtitic cells that way they can activate Th and B cells. SOme cause too powerful of a inflamatory response safe for humans

Question 19

D) What is poliomyelitis?

Answer 19

paralytic disease

Question 20

1) What was the Salk vaccine? What was the drawback?

Answer 20

Salk vaccine: inactivated viruses of the three strains. requires a series of injections.

Question 21

2) What were the advantages and disadvantages of the Sabin vaccine?

Answer 21

Sabin is administered orally, atttenuated. It can mutate and become virulent. has tobe given in 3 doses

Question 22

3) How was polio eradicated from the United States?

Answer 22

via vaccines

Question 23

E) Which childhood diseases are easily prevented through vaccination? [Table 18.3]

Answer 23

measles, mumps, small pox, diptheria, pertusis(whooping cough), paralytic poliomyetis, rubella, Haemophilus influenzae

Question 24

F) What types of vaccines are currently being researched and studied?

Answer 24

peptide, heat stable vaccines
edible, genes encoded key antigens from infectious agents to plants
and DNA based, segments of naked dna

Question 25

G) What diseases are new or improved vaccines being sought for? [Table 18.4]

Answer 25

HIV, Malaria, Influenza, strep, genital herpes, hept C, canccer

Question 26

H) What are immunoassays

Answer 26

using the specificity of antibldy- antigen reactions and using them for diagnosis. ie. syphilis- antigen binds to the causitive bacteria, Treponema pallidum. so you take juices from lesion and then put the bacteria in… if it clumps it is a positive.

Question 27

A) What does it mean to be seronegative and seropositive?

Answer 27

neg: lacks antibodies against microbe in serum
pos: has antibodies against microbe in serum

Question 28

1) What is seroconversion?

Answer 28

change from sero neg to pos

Question 29

B) What is serum?

Answer 29

fluid portion of blood that remains after blood clots

Question 30

C) What is plasma?

Answer 30

fluid portion of blood that has anticooagulant added to it

Question 31

D) What does the study of serology cover?

Answer 31

the interaction between antibodies and antigens

Question 32

E) How do you create polyclonal antibodies? What are some problems with there use?

Answer 32

The are from the serum of animals that have been vacinated. Some may bind to closely related organisms and give a false positive.

Question 33

1) What are anti-human IgG antibodies?

Answer 33

bind to a certain region on human IgG molecules

Question 34

F) What are monoclonal antibodies? How are they obtained? How can they be “humanized’?[Per. 18.1]

Answer 34

they bind to a single epitope and are manufactured.
They are created by taking b cells from an animal (short lived) and then fuseing them with other cells that will divide in the culture. They are humanised by using recombinant techniques to make the antibody more like a humans so it is less likely for the body to get rid of it.

Question 35

G) How do you determine the concentration of antibodies in a specimen?

Answer 35

You do a serological test. In this you make sequential certian dilutions of the antibodies and then you take that and put antigen into it

Question 36

1) What is the titer?

Answer 36

is the last concentration that provided evidence of a antibody antigen reaction.

Question 37

H) How are serology test done? [Figure 18.4]

Answer 37

can be done in tubes, but requires a lot

or with a microtiter

Question 38

A) What happens when antibodies bind to soluble antigens? [Figure 18.5]

Answer 38

they cross link to form insoluable lattice like complexes.

Question 39

B) What are precipitation reactions?

Answer 39

reactions in which the antibodies and antigens form a precipitate.

Question 40

1) What is the Ouchterlony technique and what is it used for? [Figure 18.6]

Answer 40

for determining precipitate reactions. This is when wells are cut in a petri dish and then filled with an antibody another an antigen so they can difuse. if not you can get the wrong antibody antigen reaction which results in a false negative.

Question 41

C) What is the difference between agglutination and precipitation reactions? [Agglutination and Precipitation video]

Answer 41

Agglutination:large insoluable particles that cross link and form latice like strucures

Question 42

1) How is a direct agglutination test done? [Figure 18.7]

Answer 42

antibody suspension is mixed with the insoluable antigen like rbs, or bacteria. If they bind together they clump together= positive results

Question 43

2) How is a passive agglutination test done? [Figure 18.8]

Answer 43

when antigens or antibodies are bound to a latex bead to make the agglutination results more visible.

Question 44

A) What can labeled antibodies be used to test for? [Figure 18.9]

Answer 44

can be used in direct or inderect tests to find specific antigens and antibodies

Question 45

1) How are direct tests done?

Answer 45

when antigen is unknown: the antigen is secured to solid surface then add labeled antibodies for specific antigen and see if they bind to eachother by rinsing the loose antibodies off

Question 46

2) How are indirect tests done?

Answer 46

antigen known: it is secured to surface. Then the patients antibodies are added. They bind and then rinse off the excess. Then add secondary antibodies ( anti human Ig G molecules that bind to the human antibodies)

Question 47

B) What is the fluorescent antibody test used for and how is it done? [Figure 18.10]

Answer 47

different antibodies are given a specific colored dye. These are added to a plate fixed with antigens.

Question 48

C) What is the enzyme-linked immunosorbent assay used for? [Figure 18.11 and ELISA video]

Answer 48

use a antibody with a enzyme attatched and then you add a substrate which will bind to the enzyme making the antibody antigen visible due to a color change.

Question 49

1) What are the differences between the direct and indirect ELISA? [Figure 18.12]
D) How do you use the Western blotting technique? [Figure 18.3]

Answer 49

Direct: Antibodies attached to a surface and then unknown antigens added
Indirect: have antigens attached to look for the antibodies
Western blotting technique: helps in determining wich protiens on antigens are reacting with antibodies. electrophoriesis is used to seperate the different sized protiens that make a specific antigen. These are fixed to a plate and patients antibodies are added to see if they will react. then a anti human IgG antibody that is florescently tagged is added

Question 50

E) How does flow cytometry count cells?

Answer 50

measures light scattered when a laser is passed over it.

Question 51

1) What can the fluorescence-activated cell sorter do?

Answer 51

is used to count different labeled florescent antibodies