Formative Assessment Flashcards

1
Q

How do DCs mature?

A

Maturation caused by microbial products/inflammatory cytokines/ damaged host cells
-> migrate to lymph nodes and present antigenic peptides to T cells

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2
Q
How are the following identified?
Helper T cells
B cells
Macrophages
Endothelial cells
Lymph vessels
A
CD4: Helper T cells
B220: B cells
F4/80, CD169: macrophages
ERTR7: endothelial cells
Lyve-1: lymph vessels
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3
Q

Describe the structure of a lymph node

A
  • Subcapsular sinus- between capsule and cortex- afferent lymph draining
  • Cortex- mainly B cells, B cell follicles (outer cortex)
  • Paracortex- inner cortex- mainly T cells
  • Medulla- blood vessels/macrophages, plasma cells- lymph flows out to efferent lymphatics
  • IFA interfollicular area- afferent lymphatics, entry of DCs
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4
Q

Outline DC subsets

A

• Can be classical (CDC, CDC11c+) or plasmocytoid (pDC)- looks more like plasma cell
• Different CDC subsets express different surface receptors (Eg CD103 in gut)
- CDC1 express XCR1+ and are cross-priming
- CDC2 express CD11b+ and are CD4 priming
• pDC- type I interferon production, antiviral function

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5
Q

Outline cross-presentation

A

Exogenous proteins from the endosome enter the cytosol and are presented in MHC I via proteasome- allows uninfected DC to still present in MHC class I to CD8- allows recognition of viruses that could interfere with MHC I presentation

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6
Q

Describe flow cytometry

A
  • Monoclonal Antibodies against particular surface molecules are conjugated to fluorescent label/dye/fluorochrome
  • Flow cytometer- measures intensity of fluorescence of each cell
  • Using isotype controls distinguish positive and negative populations for each marker
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7
Q

What do Forward scatter (FSC) and Side scatter (SSC) do?

A

Allow us to know the differentiation of different types of cells

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8
Q

What do glow cytometry histograms do?

A

To determine whether two populations are different to each other

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9
Q

How can we identify antigen specific cells using FC?

A
  • Intracellular staining- activate cells with antigen to see which cells produce cytokines- these are antigen specific
  • Tetramer/multimeter staining- peptide that is recognised by specific T cell is attached to fluorochrome
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10
Q

How can Fc measure proliferation?

A

Cells lose fluorescence as they proliferate- by measuring fluorescence intensity we can determine level of proliferation

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11
Q

How is Diptheria toxin used?

A
  • Use a tissue specific enhancer/promoter with DT receptor (microinjection to fertilised eggs)
  • Can knockout chosen cell population by injection of DT
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12
Q

What are conditional gene knockouts?

A
  • Technique to eliminate specific gene in certain tissue/cell type (inducible eg Tamoxifen)
  • Control where and when gene is knocked out to avoid embryonic mortality, to elucidate role of gene
  • eg CRE system
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13
Q

Outline CRE-Lox recombination

A

Site specific recombination:
• LoxP sequences contain specific binding sites for Cre
• Specific DNA sequence is spliced using Cre recombinase
• Floxed mouse has LoxP gene either side of target gene
• Cell specific promoters used to control Cre-> in cells with active Cre recombinase the target gene function is disrupted

Eg.
• Infar1^flox/flox: LoxP (flox) sequences in INFR1 gene
• Itgax-CRE: Cre under control of CD11c promoter
-> Cre expressed in DCs expressing CD11c
-> INFR1 knocked out in DCs expressing CD11c

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