Formative Assessment Flashcards
How do DCs mature?
Maturation caused by microbial products/inflammatory cytokines/ damaged host cells
-> migrate to lymph nodes and present antigenic peptides to T cells
How are the following identified? Helper T cells B cells Macrophages Endothelial cells Lymph vessels
CD4: Helper T cells B220: B cells F4/80, CD169: macrophages ERTR7: endothelial cells Lyve-1: lymph vessels
Describe the structure of a lymph node
- 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
Outline DC subsets
• 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
Outline cross-presentation
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
Describe flow cytometry
- 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
What do Forward scatter (FSC) and Side scatter (SSC) do?
Allow us to know the differentiation of different types of cells
What do glow cytometry histograms do?
To determine whether two populations are different to each other
How can we identify antigen specific cells using FC?
- 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
How can Fc measure proliferation?
Cells lose fluorescence as they proliferate- by measuring fluorescence intensity we can determine level of proliferation
How is Diptheria toxin used?
- Use a tissue specific enhancer/promoter with DT receptor (microinjection to fertilised eggs)
- Can knockout chosen cell population by injection of DT
What are conditional gene knockouts?
- 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
Outline CRE-Lox recombination
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
