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252 lines
10 KiB
YAML
252 lines
10 KiB
YAML
---
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# Protocol metadata
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id: PROT-0014
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name: RNA Immunoprecipitation qPCR Protocol
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version: 1.0
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description: Protocol for RNA immunoprecipitation followed by RT-qPCR to detect RNA-protein interactions
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author: Jordan Lab
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created: 2025-05-06
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last_updated: 2025-05-07
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category: molecular-biology
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# Materials required
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materials:
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- name: Cell culture dishes
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type: 10-cm or 15-cm dishes
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notes: Depending on protein/RNA abundance
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- name: PBS (cold)
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temperature: 4°C
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storage: Room temperature
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- name: UV crosslinker
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wavelength: 254 nm
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alternative: Formaldehyde crosslinking
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- name: Lysis buffer
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components: "Non-denaturing buffer with RNase inhibitors"
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storage: Prepare fresh or store at -20°C
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- name: Protein A/G beads
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preparation: Pre-blocked with BSA and tRNA
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storage: 4°C
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- name: Antibodies for target protein
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dilution: As recommended for IP
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storage: -20°C
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- name: IgG control antibody
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use: Negative control
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storage: -20°C
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- name: Glycine solution
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concentration: 2.5 M (for formaldehyde quenching)
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storage: Room temperature
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- name: RNA isolation reagents
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type: TRIzol or column-based kit
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storage: According to manufacturer's instructions
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- name: RT-qPCR reagents
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components: "Reverse transcription kit, qPCR master mix, primers"
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storage: -20°C
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# Equipment required
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equipment:
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- name: UV crosslinker
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settings: 150-300 mJ/cm²
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alternative: Formaldehyde crosslinking setup
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- name: Refrigerated centrifuge
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settings: Various speeds, 4°C
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- name: Rotating mixer
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temperature: 4°C
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- name: Thermocycler
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use: RT-qPCR and crosslink reversal
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- name: qPCR instrument
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use: Target RNA detection
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# Protocol steps - General workflow
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steps:
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- step: 1
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action: "Grow cells to desired confluency"
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details: "80-90% confluency recommended for optimal yield"
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- step: 2
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action: "Perform crosslinking"
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details: "Choose between UV or formaldehyde crosslinking methods (see detailed workflows below)"
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- step: 3
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action: "Harvest and lyse cells"
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details: "Use buffer with RNase inhibitors; keep samples cold"
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- step: 4
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action: "Pre-clear lysates"
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details: "Incubate with protein A/G beads alone for 1 hour at 4°C to reduce nonspecific binding"
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- step: 5
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action: "Perform immunoprecipitation"
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details: "Add specific antibody, incubate, then add protein A/G beads"
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- step: 6
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action: "Wash beads"
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details: "Multiple washes with increasing stringency to remove non-specific binding"
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- step: 7
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action: "Reverse crosslinks if needed"
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details: "UV: proteinase K digestion; formaldehyde: heat treatment (65°C)"
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- step: 8
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action: "Isolate RNA"
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details: "Extract RNA from immunoprecipitated complex using TRIzol or column-based kit"
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- step: 9
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action: "Perform RT-qPCR"
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details: "Reverse transcribe RNA and quantify target RNA enrichment"
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# UV crosslinking workflow
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uv_crosslinking_workflow:
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- step: 1
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action: "Grow cells to desired confluency in culture dishes"
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details: "Use 10-15 cm dishes for sufficient material"
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- step: 2
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action: "Wash cells with cold PBS"
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details: "Remove media and serum proteins; keep cells on ice to minimize RNase activity"
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- step: 3
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action: "Add fresh cold PBS"
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details: "Add enough to cover the cells but minimize UV light absorption"
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- step: 4
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action: "Perform UV crosslinking"
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details: "Use UV 254 nm at 150-300 mJ/cm²; optimize for your protein of interest"
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- step: 5
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action: "Harvest cells"
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details: "Scrape or gently trypsinize cells and collect by centrifugation"
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- step: 6
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action: "Lyse cells"
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details: "Use mild conditions suitable for maintaining RNP complexes"
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- step: 7
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action: "Pre-clear lysates"
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details: "Incubate with protein A/G beads alone to reduce nonspecific binding"
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- step: 8
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action: "Perform immunoprecipitation"
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details: "Add the specific antibody, followed by protein A/G beads"
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- step: 9
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action: "Wash beads"
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details: "Multiple washes with increasing stringency"
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- step: 10
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action: "Digest and extract RNA"
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details: "Treat with proteinase K and extract RNA"
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- step: 11
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action: "Perform RT-qPCR"
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details: "Reverse transcribe and perform qPCR to detect target RNAs"
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# Formaldehyde crosslinking workflow
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formaldehyde_crosslinking_workflow:
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- step: 1
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action: "Grow cells to desired confluency"
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details: "Use 10-15 cm dishes for sufficient material"
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- step: 2
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action: "Prepare formaldehyde solution"
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details: "Prepare fresh formaldehyde at working concentration (often 1% final in culture medium)"
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- step: 3
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action: "Crosslink cells"
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details: "Add formaldehyde directly to cells and incubate for 5–10 minutes at RT or 37°C"
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- step: 4
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action: "Quench reaction"
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details: "Add glycine (125 mM final) for 5–10 minutes to quench formaldehyde"
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- step: 5
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action: "Wash cells"
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details: "Wash thoroughly with cold PBS to remove formaldehyde"
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- step: 6
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action: "Harvest cells"
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details: "Scrape cells carefully and collect by centrifugation"
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- step: 7
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action: "Lyse cells"
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details: "Use conditions that preserve protein-RNA complexes"
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- step: 8
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action: "Perform immunoprecipitation"
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details: "Use specific antibody against protein of interest"
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- step: 9
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action: "Wash beads"
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details: "Multiple washes to remove nonspecific material"
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- step: 10
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action: "Reverse crosslink"
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details: "Heat at 65°C for several hours with SDS/high salt"
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- step: 11
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action: "Isolate RNA"
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details: "Extract RNA from immunoprecipitated sample"
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- step: 12
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action: "Perform RT-qPCR"
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details: "Reverse transcribe and quantify targets by qPCR"
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# Critical parameters
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critical_parameters:
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- parameter: "Crosslinking method selection"
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details: "UV is more specific for direct interactions; formaldehyde captures larger complexes"
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- parameter: "Antibody specificity"
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details: "Validate antibody IP efficiency by Western blot before RIP"
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- parameter: "RNase control"
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details: "Use RNase inhibitors in all buffers and work quickly at 4°C"
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- parameter: "Wash stringency"
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details: "Balance between removing background and maintaining specific interactions"
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# Troubleshooting
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troubleshooting:
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- problem: "Poor RNA yield"
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solution: "Increase starting material; optimize crosslinking conditions; check for RNase contamination"
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- problem: "High background in control IPs"
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solution: "Increase wash stringency; pre-block beads with BSA/tRNA; use more specific antibody"
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- problem: "No enrichment of target RNA"
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solution: "Verify protein-RNA interaction using alternative approach; check crosslinking efficiency; try different antibody"
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# Method comparisons
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considerations:
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uv_crosslinking:
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- advantage: "Standardize irradiation distance/energy for reproducibility"
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- advantage: "More specific crosslinks between directly interacting residues"
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- advantage: "Better for pinpointing precise binding sites"
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- disadvantage: "Requires specialized equipment (UV crosslinker)"
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- disadvantage: "May damage RNA integrity at high doses"
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- note: "More common in CLIP-based methods for precise interaction mapping"
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formaldehyde_crosslinking:
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- advantage: "Straightforward chemical method without specialized equipment"
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- advantage: "Captures indirect interactions within larger complexes"
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- advantage: "Often higher yield"
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- disadvantage: "Higher background from nonspecific crosslinks"
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- disadvantage: "Reversal requires potentially harsh conditions (heating, high salt)"
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- note: "Better for detecting weak or transient interactions"
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# Safety considerations
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safety:
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ppe: "Lab coat, gloves, and eye protection required"
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hazards: "UV radiation: avoid direct exposure; Formaldehyde: toxic and carcinogenic, use in fume hood"
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waste: "Dispose of crosslinking reagents according to institutional guidelines"
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# Quality control
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quality_control:
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- check: "Include IgG control IP"
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criteria: "Should show minimal enrichment of target RNAs"
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- check: "Include input RNA sample"
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criteria: "For normalization and calculating percent input"
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- check: "Test known RNA-protein interaction"
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criteria: "Should show significant enrichment over IgG control"
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# Data analysis
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data_analysis:
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- step: 1
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action: "Calculate fold enrichment"
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details: "Compare target RNA in specific IP vs. IgG control IP"
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- step: 2
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action: "Calculate percent input"
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details: "Compare RNA abundance in IP vs. a defined percentage of input material"
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- step: 3
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action: "Statistical analysis"
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details: "Perform appropriate statistical tests on biological replicates"
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# Best practices
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best_practices:
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- "Run pilot experiments to optimize crosslinking conditions for specificity vs. yield"
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- "Test different crosslinking strengths and confirm with a known positive RNA target"
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- "Include IgG control or nonspecific antibody to measure background binding"
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- "Use input RNA to normalize or calculate percentage of input in qPCR"
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- "If possible, use a known RNA-protein interaction as positive control"
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- "Incorporate RNase inhibitors in all buffers and keep samples cold"
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- "For many RIP-qPCR experiments, mild UV crosslinking at 254 nm is preferred"
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# References
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references:
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- "Peritz T, et al. (2006) Immunoprecipitation of mRNA-protein complexes. Nat Protoc. 1(2):577-580"
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- "Keene JD, et al. (2006) RIP-Chip: the isolation and identification of mRNAs, microRNAs and protein components of ribonucleoprotein complexes from cell extracts. Nat Protoc. 1(1):302-307"
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- "Niranjanakumari S, et al. (2002) Reversible cross-linking combined with immunoprecipitation to study RNA-protein interactions in vivo. Methods. 26(2):182-190"
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# Notes
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notes: |
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- Two crosslinking methods are described: UV (254 nm) and formaldehyde
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- UV crosslinking is more specific but requires specialized equipment
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- Formaldehyde crosslinking is simpler but may have higher background
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- Always include appropriate controls (IgG, input RNA)
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- Consider CLIP-based methods for more precise mapping of binding sites
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- For studying RNA binding proteins that interact with many targets, consider combining with RNA-seq (RIP-seq)
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