Studying RNA Interactors of Protein Kinase RNA-Activated during the Mammalian Cell Cycle

Sujin Kim; Minjeong Kang; Yoosik Kim

doi:10.3791/59215

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W tym Artykule

Podsumowanie
Streszczenie
Wprowadzenie
Protokół
Wyniki
Dyskusje
Ujawnienia
Podziękowania
Materiały
Odniesienia
Przedruki i uprawnienia

Podsumowanie

We present experimental approaches for studying RNA-interactors of double-stranded RNA binding protein kinase RNA-activated (PKR) during the mammalian cell cycle using HeLa cells. This method utilizes formaldehyde to crosslink RNA-PKR complexes and immunoprecipitation to enrich PKR-bound RNAs. These RNAs can be further analyzed through high-throughput sequencing or qRT-PCR.

Streszczenie

Protein kinase RNA-activated (PKR) is a member of the innate immune response proteins and recognizes the double-stranded secondary structure of viral RNAs. When bound to viral double-stranded RNAs (dsRNAs), PKR undergoes dimerization and subsequent autophosphorylation. Phosphorylated PKR (pPKR) becomes active and induces phosphorylation of the alpha subunit of eukaryotic initiation factor 2 (eIF2α) to suppress global translation. Increasing evidence suggests that PKR can be activated under physiological conditions such as during the cell cycle or under various stress conditions without infection. However, our understanding of the RNA activators of PKR is limited due to the lack of a standardized experimental method to capture and analyze PKR-interacting dsRNAs. Here, we present an experimental protocol to specifically enrich and analyze PKR bound RNAs during the cell cycle using HeLa cells. We utilize the efficient crosslinking activity of formaldehyde to fix PKR-RNA complexes and isolate them via immunoprecipitation. PKR co-immunoprecipitated RNAs can then be further processed to generate a high-throughput sequencing library. One major class of PKR-interacting cellular dsRNAs is mitochondrial RNAs (mtRNAs), which can exist as intermolecular dsRNAs through complementary interaction between the heavy-strand and the light-strand RNAs. To study the strandedness of these duplex mtRNAs, we also present a protocol for strand-specific qRT-PCR. Our protocol is optimized for the analysis of PKR-bound RNAs, but it can be easily modified to study cellular dsRNAs or RNA-interactors of other dsRNA binding proteins.

Wprowadzenie

Protein kinase RNA-activated (PKR), also known as eukaryotic initiation factor 2-alpha kinase 2 (EIF2AK2), is a well-characterized protein kinase that transmits information provided by RNAs. It belongs to the eukaryotic translation initiation 2 subunit alpha (eIF2α) kinase family and phosphorylates eIF2α at serine 51 in response to infection to suppress global translation¹. In this context, PKR is activated by viral double-stranded RNAs (dsRNAs), which provide a platform for PKR dimerization and autophosphorylation². In addition to eIF2α, PKR can also phosphorylate p53, insulin receptor substrate 1, inhibitor κB, and c-Jun N-terminal kinase (JNK) to regulate activity of numerous signal transduction pathways³^,⁴^,⁵^,⁶.

PKR was originally identified as a kinase that phosphorylated eIF2α during poliovirus infection by recognizing poliovirus’ dsRNAs⁷^,⁸. PKR is increasingly found to play multifaceted roles beyond immune response, and its aberrant activation or malfunction is implied in numerous human diseases. Activated/Phosphorylated PKR (pPKR) is frequently observed during apoptosis and is a common characteristic of patients with degenerative diseases, particularly neurodegenerative diseases such as Huntington’s, Parkinson’s, and Alzheimer’s disease⁹^,¹⁰^,¹¹^,¹²^,¹³. In addition, PKR is activated under various stress conditions such as metabolic stress and heat shock¹⁴^,¹⁵^,¹⁶^,¹⁷. On the other hand, inhibition of PKR results in increased cell proliferation and even malignant transformation¹⁸^,¹⁹. PKR function is also important in normal brain function and during the cell cycle as the level of pPKR is elevated during the M phase²⁰^,²¹^,²². In this context, pPKR suppresses global translation and provides cues to key mitotic signaling systems that are required for proper cell division²⁰. Moreover, prolonged activation of PKR resulted in G2/M phase cell cycle arrest in Chinese hamster ovary cells²³. Consequently, PKR phosphorylation is regulated by the negative feedback loop to ensure rapid deactivation during M/G1 transition²¹.

Despite the wide range of PKR function, our understanding of PKR activation is limited due to the lack of a standardized high-throughput experimental approach to capture and identify dsRNAs that can activate PKR. Previous studies have shown that PKR can interact with dsRNAs formed by two inverted Alu repeats (IRAlus)²⁰^,²⁴, but the possibility of the existence of additional cellular dsRNAs that can activate PKR during the cell cycle or under stress conditions in human cells was unexplored. The conventional approach in identifying RNA-interactors of an RNA binding protein (RBP) uses UV light to crosslink RNA-RBP complexes²⁵^,²⁶^,²⁷. A recent study applied this UV crosslinking approach in a mouse system and identified that small nucleolar RNAs can regulate PKR activation during metabolic stress¹⁶. By utilizing high crosslinking efficiency of formaldehyde, we presented an alternative method to identify PKR-interacting RNAs during the cell cycle in HeLa cells²⁸. A similar approach has been applied to study other dsRBPs such as Staufen and Drosha²⁹^,³⁰^,³¹. We found that PKR can interact with various types of noncoding RNAs such as short interspersed nuclear element (SINE), long interspersed nuclear element (LINE), endogenous retrovirus element (ERV), and even alpha-satellite RNAs. In addition, we showed that PKR can interact with mitochondrial RNAs (mtRNAs), which form intermolecular dsRNAs through complementary interaction between the heavy-strand and the light strand RNAs²⁸. A recent publication further supported our data that some mtRNAs exist in a duplex form and can activate dsRNA sensors such as melanoma differentiation-associated protein 5 to induce interferons³². More importantly, the expression and subcellular localization of mtRNAs are modulated during the cell cycle and by various stressors, which may be important in their ability to regulate PKR activation²⁸.

In this article, we present a detailed protocol for a recently developed formaldehyde crosslinking and immunoprecipitation (fCLIP) method to capture and analyze PKR-interacting RNAs during the cell cycle. We demonstrate the method to prepare cell cycle arrest samples using thymidine and nocodazole. We then present the fCLIP process to isolate PKR-bound RNAs and a method to prepare high-throughput sequencing library to identify these RNAs. Furthermore, we delineate detailed procedures to analyze PKR-bound RNAs using qRT-PCR. Specifically, we present a strand-specific reverse transcription procedure to analyze the strandedness of mtRNAs. The described protocol is optimized for HeLa cells and PKR, but key steps such as the preparation of cell cycle sample, fCLIP, and strand-specific qRT-PCR analysis can be easily modified to study cellular dsRNAs or to identify RNA interactors of other dsRBPs.

Protokół

1. Solution and cell preparation

Solution preparation
1. For the cell culture medium, prepare medium for HeLa cell culture by adding 50 mL of fetal bovine serum (FBS) to 500 mL of Dulbecco’s Modified Eagle’s Medium (DMEM).
  NOTE: Antibiotics can be added to the cell culture medium, but we do not use antibiotics.
2. For the 0.1% paraformaldehyde, dissolve 4% (w/v) paraformaldehyde in 1x Phosphate-Buffered Saline (PBS) with heating on a hot plate and dilute to make 30 mL of 0.1% (v/v) paraformaldehyde by adding 1x PBS.
  CAUTION: Perform all steps in a fume hood and be careful not to boil the paraformaldehyde solution. Protect the 0.1% solution from light and store at 4 °C. Use the solution within one month.
  NOTE: The pH of the final 0.1% (v/v) paraformaldehyde solution should be around 7.
3. Prepare fCLIP lysis buffer: 20 mM Tris-HCl (pH 7.5), 15 mM NaCl, 10 mM EDTA, 0.5% (v/v) nonidet-p40 (NP-40), 0.1% (v/v) Triton X-100, 0.1% (v/v) sodium dodecyl sulfate (SDS), and 0.1% (w/v) sodium deoxycholate. Add triple distilled water (TDW) to 40 mL. Store at 4 °C.
4. Prepare fCLIP wash buffer: 20 mM Tris-HCl (pH 7.5), 150 mM NaCl, 10 mM EDTA, 0.1% (v/v) NP-40, 0.1% (v/v) Triton X-100, 0.1% (v/v) SDS, and 0.1% (w/v) sodium deoxycholate. Add TDW to 40 mL. Store at 4 °C.
5. Prepare 4x PK buffer: 400 mM Tris-HCl (pH 7.5), 200 mM NaCl, 40 mM EDTA, and 4% (v/v) SDS. Add TDW to 40 mL. Store at room temperature.
6. Prepare fCLIP elution buffer: 20 mL of 4x PK buffer, 21 g of urea, and 8.5 mL of TDW. Prepare fresh.
7. Prepare RNA elution buffer: 0.3 M NaOAc and 2% (w/v) SDS. Store at room temperature.
8. Prepare 2x RNA loading dye: 0.025% (w/v) bromophenol blue, 0.025% (w/v) xylene cyanol, 5 mM EDTA, 0.05% (w/v) SDS, and 95% (v/v) formamide. Store at -20 °C.
9. Prepare 1x TBE buffer: 0.089 M Tris-Borate and 0.002 M EDTA. Prepare 500 mL of TBE buffer.
Preparation of S or M phase-arrested cells
1. Seed ~750,000 or ~1,000,000 HeLa cells for S or M phase-arrested samples, respectively. Grow cells at 37 °C and 5% CO₂for 24 h.
2. Treat the cells with 2 mM thymidine and incubate for 18 h at 37 °C.
3. Wash the cells two times with PBS. Add fresh media and incubate for 9 h at 37 °C.
4. For S phase-arrested cells, treat cells with 2 mM thymidine. For M phase-arrested cells, treat cells with 100 ng/mL nocodazole. Incubate for 15 h at 37 °C and harvest cells.
  NOTE: The homogeneity of the cell cycle samples can be checked using FACS.

2. Formaldehyde cross-linking and immunoprecipitation

Cell harvest
1. For an S phase sample, collect cells with a cell scraper and transfer into a 15 mL conical tube. For an M phase sample, tap the side of the cell culture dish to detach M phase-arrested cells and transfer them into a 15 mL conical tube.
  NOTE: To increase the homogeneity of the M phase-arrested cells, do not use a cell scraper.
2. Centrifuge the cells at 380 x g at room temperature for 3 min. Remove the supernatant and re-suspend with 1 mL of cold PBS and transfer into a 1.5 mL microcentrifuge tube.
3. Centrifuge the cells at 10,000 x g at 4 °C for 30 s. Remove the supernatant completely.
Formaldehyde crosslinking
1. Add 750 μL of 0.1% paraformaldehyde for 10 min at room temperature to fix the cells.
2. Add 250 μL of 1 M glycine and incubate an additional 10 min at room temperature to quench the reaction. Centrifuge the cells at 10,000 x g at 4 °C for 30 s. Remove the supernatant completely.
3. Re-suspend with 1 mL of PBS. Centrifuge the cells at 10,000 x g at 4 °C for 30 s and remove the supernatant.
4. Re-suspend with 400 μL of fCLIP lysis buffer supplemented with 0.2% (v/v) protease inhibitor and 2% (v/v) RNase inhibitor. Incubate on ice for 10 min and sonicate using an ultrasonicator.
5. Add 11 μL of 5 M NaCl to adjust NaCl concentration to ~150 mM. Vortex briefly and centrifuge at 21,130 x g at 4 °C for 15 min. Transfer the supernatant to a pre-chilled 1.5 mL microcentrifuge tube.
  NOTE: Retain 40 μL of supernatant in a new centrifuge tube as the input sample. Store the input sample at 4 °C.
Immunoprecipitation
1. Add 20 μL of Protein A beads into a 1.5 mL microcentrifuge tube.
2. Wash the beads with 400 μL of fCLIP lysis buffer. Centrifuge the beads at 1,000 x g at 4 °C for 1 min. Remove the supernatant and add 400 μL of fCLIP lysis buffer carefully. Gently re-suspend the beads by inverting 3~4 times.
3. Repeat the wash step three times. After the final wash, remove the supernatant completely.
4. Re-suspend the beads in 300 μL of fCLIP lysis buffer. Add 8.3 μL of 5 M NaCl to adjust NaCl concentration to ~150 mM. Add 10 μL of PKR antibody and incubate for 3 h on a rotator at 4 °C.
5. Centrifuge the beads at 1,000 x g at 4 °C for 1 min. Remove the supernatant and add 400 μL of fCLIP wash buffer. Gently re-suspend the beads by inverting 3~4 times.
6. Repeat the wash step two times. After the final wash, remove the supernatant completely.
  NOTE: Never use a vortex mixer. Invert the tube gently with hands.
7. Add 300 μL of lysate and incubate for 3 h at 4 °C on a rotator.
  NOTE: Longer incubation time may result in increased background binding.
8. Centrifuge the beads at 1,000 x g at 4 °C for 1 min. Remove the supernatant and add 400 μL of fCLIP wash buffer. Gently re-suspend the beads by inverting 3~4 times.
9. Repeat the wash step three times. After the final wash, remove the supernatant completely.
10. Add 300 μL of fCLIP elution buffer. Incubate in a thermomixer for 3 h at 25 °C to elute PKR from the beads.
  NOTE: Prepare the fCLIP elution buffer fresh.
11. Centrifuge at 1,000 x g at room temperature and transfer the supernatant to a clean siliconized tube.
  NOTE: A microcentrifuge tube is also ok, but siliconized tube is preferred to prevent evaporation during the de-crosslinking step (step 2.3.12).
12. Add 300 μL of proteinase K (20 mg/mL) and incubate overnight at 65 °C.
  NOTE: Use a thermomixer with heated cover to avoid evaporation.
RNA extraction
1. Add 580 μL of acid-phenol chloroform and vortex for 30 s. Incubate at 37 °C for 1 h.
2. Vortex for 30 s and centrifuge at 12,000 x g at room temperature for 10 min.
3. Transfer the top layer into a clean 1.5 mL microcentrifuge tube. Add 1/10 volume of 3 M NaOAc, 0.5 μL of coprecipitant (e.g., Glycoblue), and an equal volume of isopropanol. Incubate overnight at -20 °C.
4. Precipitate pellets by centrifuging at maximum speed at 4 °C for 1 h.
  NOTE: If RNA/DNA pellets were not observed, add an additional 0.5 μL of coprecipitant and centrifuge for an additional 1 h. Continue this step until RNA/DNA pellets are observed.
5. Remove the supernatant and add 1 mL of 75% ethyl alcohol. Centrifuge at 12,000 x g at 4 °C for 5 min. Repeat the wash step one more time. Remove the supernatant completely and dry the pellet at room temperature.
6. Add 42 μL of TDW, 5 μL of DNase I buffer, 1 μL of RNase Inhibitor, and 2 μL of DNase I. Incubate at 37 °C for 1 h.
7. Add 150 μL of TDW and 200 μL of acid-phenol chloroform. Vortex for 30 s. Centrifuge at 12,000 x g at room temperature for 10 min.
8. Transfer the top layer into a clean 1.5 mL microcentrifuge tube. Add 20 μL of 3 M NaOAc, 0.5 μL of coprecipitant, and 1 mL of 100% ethyl alcohol. Incubate overnight at -80 °C.
9. Precipitate pellets and wash with 75% ethyl alcohol as described in steps 2.4.4 to 2.4.5.
10. Re-suspend in the appropriate amount of TDW.

3. Sequencing Library Preparation

rRNA removal
1. Re-suspend the RNA pellets from step 2.4.10 with 28 μL of TDW.
  NOTE: The maximum amount of total RNA should be less than 5 μg.
2. Follow the procedures provided by the rRNA removal kit’s reference guide to remove rRNA.
3. Clean up rRNA depleted RNAs by adding 160 μL of magnetic beads.
  1. Mix by pipetting ~15 times and incubate at room temperature for 15 min.
  2. Attach the tube on a magnetic bar and remove the supernatant.
  3. Add 300 μL of 80% ethyl alcohol while the beads are still attached on the magnetic bar and incubate for 30 s.
  4. Replace ethyl alcohol with a fresh 300 μL solution. Air dry the beads on the magnetic bar for 12 min at room temperature.
  5. Re-suspend the beads in 12 μL of TDW and mix by pipetting 15 times.
  6. Attach the beads on the magnetic bar and move the supernatant to a clean PCR tube.
4. Deplete the fragmented ribosomal RNAs (rRNAs) following the procedures provided by rRNA Depletion Kit.
5. Clean up the RNAs by adding 110 μL of magnetic beads and repeating steps 3.1.3.1 to 3.1.3.6.
RNA labeling and adaptor ligation
1. On rRNA-depleted RNAs, add 2 μL of 10x CIAP buffer, 1 μL of RNase inhibitor, and 2 μL of antarctic alkaline phosphatase. Incubate at 37 °C for 1 h and then at 65 °C for 5 min to inactivate the phosphatase.
2. Add 3 μL of 10x PNK buffer, 1.5 μL of RNase inhibitor, 1.5 μL of T4 PNK enzyme, 0.8 μL of r-ATP, and 1.7 μL of TDW. Incubate at 37 °C for 50 min.
3. Add 1.5 μL of 10 mM ATP and incubate at 37 °C for additional 40 min.
4. Stop the reaction by adding 170 μL of the RNA elution buffer.
5. Add 200 μL of acid-phenol chloroform and vortex for 30 s. Centrifuge at 12,000 x g at room temperature for 10 min.
6. Transfer the top layer into a clean 1.5 mL microcentrifuge tube. Add 20 μL of 3 M NaOAc, 0.5 μL of coprecipitant, and 1 mL of 100% ethyl alcohol. Incubate overnight at -80 °C.
7. Precipitate RNA pellets and wash with 75% ethyl alcohol as described in steps 2.4.4 to 2.4.5. Re-suspend in 4.5 μL of TDW and add 9 μL of 2x RNA loading dye.
8. Heat the sample at 95 °C for 5 min and load on a 10% Urea-PAGE gel.
9. Run the gel at 370 V for 40 min.
  NOTE: Pre-run the gel at 370 V for 90 min before loading the sample.
10. Cut the gel at the ~100 – 500 nucleotide region and break the gel.
11. Add 700 μL of 0.3 M NaCl and incubate overnight at 4 °C on a rotator.
12. Transfer the solution to a column and centrifuge at maximum speed at room temperature for 5 min.
13. Transfer the eluate into a clean 1.5 mL microcentrifuge tube. Add 1/10 volume of 3 M NaOAc, 0.5 μL of coprecipitant, and an equal volume of isopropanol. Incubate overnight at -20 °C.
3' adaptor ligation
1. Precipitate RNA pellets and wash with 75% ethyl alcohol as described in steps 2.4.4 to 2.4.5.
2. Re-suspend the RNA pellets in 6.5 μL of TDW and add 1 μL of 10 μM 3' adaptor.
3. Transfer the solution to a PCR tube and incubate at 70 °C for 2 min.
4. Add 1 μL of 10x ligation buffer, 0.5 μL of RNase inhibitor, and 1 μL of T4 RNA ligase 2. Incubate at 28 °C for 1 h, 25 °C for 6 h, and 22 °C for 6 h.
5. Add 12 μL of 2x RNA loading dye and heat at 95 °C for 5 min.
6. Gel purify the 3' adaptor ligated RNAs as described in 3.2.9 to 3.2.13.
5' adaptor ligation
1. Precipitate RNA pellets and wash with 75% ethyl alcohol as described in steps 2.4.4 to 2.4.5.
2. Re-suspend the RNA pellets in 4.2 μL of TDW and add 1 μL of 5 μM 5' adaptor.
3. Transfer the solution to a PCR tube and incubate at 70 °C for 2 min.
4. Add 0.8 μL of 10x ligase buffer, 0.4 μL of RNase inhibitor, 0.8 μL of 10 mM ATP, 0.8 μL of T4 RNA ligase 1. Incubate at 28 °C for 1 h, 25 °C for 6 h, and 22 °C for 6 h.
Reverse transcription and PCR amplification
1. On 5’ adaptor ligated RNAs, add 1 μL of 4 μM reverse transcription primer. Incubate at 70 °C for 2 min and immediately cool to 4 °C.
2. Add 4 μL of 5x FS buffer, 4 μL of 2.5 mM dNTP, 1 μL of 0.1 M DTT, 1 μL of RNase inhibitor, and 1 μL of reverse transcriptase. Incubate at 50 °C for 1 h and 70 °C for 15 min.
3. Prepare PCR amplification
  1. Mix 1 μL of RT product, 1 μL of 25 μM RPI primer, 1 μL of 25 μM RP1 primer, 10 μL of 5x HF buffer, 4 μL of 2.5 mM dNTP, 32.5 μL of TDW, and 0.5 μL of high-fidelity polymerase.
  2. Run PCR program for 11~13 cycles.
    NOTE: The program for the PCR is: 98 °C for 30 s for a hot start, 98 °C for 10 s, 60 °C for 30 s and 72 °C for 45 s for amplification, and 72 °C for 5 min. The amplification step is repeated for 11-13 cycles.
4. Clean up the PCR products using 40 μL of the magnetic beads and following steps 3.1.3.1 to 3.1.3.6 but using 10 μL of TDW to elute the DNA.
5. Add 2 μL of 10x DNA loading dye. Load the sample on a 6% acrylamide gel and run at 200 V for 30 min.
6. Stain with Sybr gold (0.01% (v/v) in 1x TBE buffer) for 5 min at room temperature.
7. De-stain in 1x TBE buffer for 5 min at room temperature.
8. Cut the gel at the ~200 – 700 nucleotide region and break the gel.
9. Add 700 μL of 0.3 M NaCl and incubate overnight at room temperature to elute the DNA.
10. Load everything onto a column and centrifuge at maximum speed at room temperature for 5 min.
11. Transfer the eluate into a clean 1.5 mL microcentrifuge tube. Add 1/10 volume of 3 M NaOAc, 0.5 μL of coprecipitant, and an equal volume of isopropanol. Incubate overnight at -20 °C.
12. Precipitate DNA pellets and wash with 75% ethyl alcohol as described in steps 2.4.4 to 2.4.5. Re-suspend in 20 μL of TDW.
13. Analyze the sample using a sequencer.

4. Analysis of PKR-interacting RNAs using qRT-PCR

Method 1: Random hexamer reverse transcription
1. Re-suspend RNA pellets from step 2.4.10 with 8.5 μL of TDW and transfer the solution to a PCR tube.
2. Add 0.5 μL of 100 μM random hexamers and 4 μL of 2.5 mM dNTP mix.
3. Heat the solution at 65 °C for 5 min and immediately incubate on ice for at least 1 min.
4. Make the reaction mix: 4 μL of 5x SSIV buffer, 1 μL of 100 mM DTT, 1 μL of RNase Inhibitor, and 1 μL of reverse transcriptase (200 U/μL). Add the reaction mix to the RNA solution.
5. Incubate the mixture at 23 °C for 10 min, 50 °C for 10 min, and 80 °C for 10 min.
6. Analyze the cDNA using a real-time PCR system.
  NOTE: The program for the real-time PCR is: 95 °C for 3 min for hot start, 95 °C for 5 s and 60 °C for 10 s for amplification, and 95 °C for 30 s, 65 °C for 30 s, and 95 °C for 30 s for melt. The amplification step is repeated for 40 cycles.
Method 2: Strand-specific reverse transcription
1. Prepare a master mix of reverse primers: Mix equal amounts of gene specific reverse transcription primers containing CMV promoter sequence followed by ~20 nucleotides of gene specific sequences.
  NOTE: The combined concentration of all gene specific RT primers is 4 μM.
2. Re-suspend RNA pellets from step 2.4.10 with 8.5 μL of TDW and transfer the solution to a PCR tube.
3. Add 0.5 μL of 4 μM master mix of reverse transcription primers and 4 μL of 2.5 mM dNTP mix.
4. Heat the solution at 65 °C for 5 min and immediately incubate on ice for at least 1 min.
5. Prepare the reaction solution by mixing 4 μL of 5x SSIV buffer, 1 μL of 100 mM DTT, 1 μL of RNase Inhibitor, and 1 μL of reverse transcriptase (200 U/μL). Add the reaction solution to the RNA-primer mix.
6. Incubate the solution at 50 °C for 10 min and 80 °C for 10 min.
7. Analyze the cDNA using the real-time PCR system.
  NOTE: The program for the real-time PCR is same as the one described in Method 1.

Wyniki

A schematic for the process to arrest HeLa cells at the S or M phase of the cell cycle is shown in Figure 1. For an M phase-arrested sample, we can clearly visualize round shaped cells under the microscope (Figure 2A). To examine the efficiency of the cell cycle arrest, the nuclear content of the cell can be analyzed using FACS (Figure 2B). Figure 3 shows representative data for immunoprecipitation efficiency test, where ...

Dyskusje

The process to prepare S or M phase-arrested samples is illustrated in Figure 1. To arrest cells at the S phase, we used a thymidine double block method where we treated cells with thymidine two times with a 9 h release in between to ensure high arrest efficiency (Figure 1A). For M phase arrest, we treated cells once with thymidine followed by a 9 h release and then applied nocodazole to block cells at prometaphase (Figure 1B). One ...

Ujawnienia

The authors have nothing to disclose.

Podziękowania

This work was supported by Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Korean government Ministry of Science and ICT (NRF-2016R1C1B2009886).

Materiały

Name	Company	Catalog Number	Comments
0.5 M EDTA, pH 8.0	Thermo Fisher Scientific	AM9260G
1 M Tris, pH 7.0	Thermo Fisher Scientific	AM9855G
1 M Tris, pH 8.0	Thermo Fisher Scientific	AM9855G
1.7 mL microcentrifuge tube	Axygen	MCT-175-C
10% Nonidet-p40 (NP-40)	Biosolution	BN015
10X DNA loading buffer	TaKaRa	9157
15 mL conical tube	SPL	50015
3' adaptor			5'-rApp NN NNT GGA ATT CTC GGG TGC CAA GG/3ddC/-3'
3 M Sodium Acetate pH 5.5	Thermo Fisher Scientific	AM9740
5' adaptor			5'-GUU CAG AGU UCU ACA GUC CGA CGA UCN NNN-3'
5 M NaCl	Thermo Fisher Scientific	AM9760G
50 mL conical tube	SPL	50050
Acid-phenol chloroform, pH 4.5	Thermo Fisher Scientific	AM9722
Agencourt AMPure XP	Beckman Coulter	A63881	Magnetic beads DNA/RNA clean up
Antarctic alkaline phosphatase	New England Biolabs	M0289S
Anti-DGCR8			Made in house
Anti-PKR (D7F7)	Cell signaling technology	12297S
Anti-PKR (Milli)	Millipore EMD	07-151
ATP (100 mM)	GE Healthcare	GE27-2056-01
Bromophenol blue sodium salt	Sigma-aldrich	B5525
Calf intestinal alkaline phosphatase	TaKaRa	2250A
Cell scraper 25 cm 2-position	Sarstedt	83.183
CMV promoter sequence			5'-CGCAAATGGGCGGTAGGCGTG-3'
Dulbecco's modified eagle medium	Welgene	LM001-05
dNTP mixture (2.5 mM)	TaKaRa	4030
Ethanol, Absolute, ACS Grade	Alfa-Aesar	A9951
Fetal bovine serum	Merck	M-TMS-013-BKR
Formamide	Merck	104008
Glycine	Bio-basic	GB0235
GlycoBlue coprecipitant (15 mg/mL)	Thermo Fisher Scientific	AM9516
Isopropanol	Merck	8.18766.1000
NEBNext rRNA Depletion Kit	New England Biolabs	E6318	rRNA Depletion Kit
Nocodazole	Sigma-Aldrich	M1404
Normal rabbit IgG	Cell signaling technology	2729S
Paraformaldehyde	Sigma-Aldrich	6148
PCR forward primer (RP1)			5'-AAT GAT ACG GCG ACC ACC GCG ATC TAC ACG TTC AGA GTT CTA CAG TCC GA-3'
PCR index reverse primer (RPI)			5'-CAA GCA GAA GAC GGC ATA CGA GAT NNN NNN GTG ACT GGA GTT CCT TGG CAC CCG AGA ATT CCA-3'
PCR tubes with flat cap, 0.2 mL	Axygen	PCR-02-C
Phosphate bufered saline (PBS) Tablet	TaKaRa	T9181
Phusion high-fidelity DNA polymerase	New England Biolabs	M0530	High-fidelity polymerase
PlateFuge microcentrifuge with swing-out rotor	Benchmark	c2000
Polynucleotide kinase (PNK)	TaKaRa	2021A
Proteinase K, recombinant, PCR Grade	Sigma-Aldrich	3115879001
qPCR primer sequence: CO1 Heavy			Forward/Reverse: 5′-GCCATAACCCAATACCAAACG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CO1 Light			Forward/Reverse: 5′-TTGAGGTTGCGGTCTGTTAG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CO2 Heavy			Forward/Reverse: 5′-CTAGTCCTGTATGCCCTTTTCC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CO2 Light			Forward/Reverse: 5′-GTAAAGGATGCGTAGGGATGG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CO3 Heavy			Forward/Reverse: 5′-CCTTTTACCACTCCAGCCTAG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CO3 Light			Forward/Reverse: 5′-CTCCTGATGCGAGTAATACGG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CYTB Heavy			Forward/Reverse: 5′-CAATTATACCCTAGCCAACCCC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: CYTB Light			Forward/Reverse: 5′-GGATAGTAATAGGGCAAGGACG -3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: GAPDH			Forward/Reverse: 5′-CAACGACCACTTTGTCAAGC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND1 Heavy			Forward/Reverse: 5′-TCAAACTCAAACTACGCCCTG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND1 Light			Forward/Reverse: 5′-GTTGTGATAAGGGTGGAGAGG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND4 Heavy			Forward/Reverse: 5′-CTCACACTCATTCTCAACCCC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND4 Light			Forward/Reverse: 5′-TGTTTGTCGTAGGCAGATGG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND5 Heavy			Forward/Reverse: 5′-CTAGGCCTTCTTACGAGCC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND5 Light			Forward/Reverse: 5′-TAGGGAGAGCTGGGTTGTTT-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND6 Heavy			Forward/Reverse: 5′-TCATACTCTTTCACCCACAGC-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
qPCR primer sequence: ND6 Light			Forward/Reverse: 5′-TGCTGTGGGTGAAAGAGTATG-3′/5′-CGCAAATGGGCGGTAGGCGTG-3′
Random hexamer	Thermo Fisher Scientific	SO142
Recombinant Dnase I (Rnase-free) (5 U/μL)	TaKaRa	2270A
Recombinant Rnase inhibitor (40 U/μL)	TaKaRa	2313A
Ribo-Zero rRNA Removal Kit	Illumina	MRZH116	rRNA Removal Kit
Rotator	FINEPCR, ROTATOR AG	D1.5-32
RT primer sequence: CO1 Heavy			5′-CGCAAATGGGCGGTAGGCGTGTTGAGGTTGCGGTCTGTTAG-3′
RT primer sequence: CO1 Light			5′-CGCAAATGGGCGGTAGGCGTGGCCATAACCCAATACCAAACG-3′
RT primer sequence: CO2 Heavy			5′-CGCAAATGGGCGGTAGGCGTGGTAAAGGATGCGTAGGGATGG-3′
RT primer sequence: CO2 Light			5′-CGCAAATGGGCGGTAGGCGTGCTAGTCCTGTATGCCCTTTTCC-3′
RT primer sequence: CO3 Heavy			5′-CGCAAATGGGCGGTAGGCGTGCTCCTGATGCGAGTAATACGG-3′
RT primer sequence: CO3 Light			5′-CGCAAATGGGCGGTAGGCGTGCCTTTTACCACTCCAGCCTAG-3′
RT primer sequence: CYTB Heavy			5′-CGCAAATGGGCGGTAGGCGTGGGATAGTAATAGGGCAAGGACG-3′
RT primer sequence: CYTB Light			5′-CGCAAATGGGCGGTAGGCGTGCAATTATACCCTAGCCAACCCC-3′
RT primer sequence: GAPDH			5′-CGCAAATGGGCGGTAGGCGTGTGAGCGATGTGGCTCGGCT-3′
RT primer sequence: ND1 Heavy			5′-CGCAAATGGGCGGTAGGCGTGGTTGTGATAAGGGTGGAGAGG-3′
RT primer sequence: ND1 Light			5′-CGCAAATGGGCGGTAGGCGTGTCAAACTCAAACTACGCCCTG-3′
RT primer sequence: ND4 Heavy			5′-CGCAAATGGGCGGTAGGCGTGTGTTTGTCGTAGGCAGATGG-3′
RT primer sequence: ND4 Light			5′-CGCAAATGGGCGGTAGGCGTGCCTCACACTCATTCTCAACCC-3′
RT primer sequence: ND5 Heavy			5′-CGCAAATGGGCGGTAGGCGTGTTTGGGTTGAGGTGATGATG-3′
RT primer sequence: ND5 Light			5′-CGCAAATGGGCGGTAGGCGTGCATTGTCGCATCCACCTTTA-3′
RT primer sequence: ND6 Heavy			5′-CGCAAATGGGCGGTAGGCGTGGGTTGAGGTCTTGGTGAGTG-3′
RT primer sequence: ND6 Light			5′-CGCAAATGGGCGGTAGGCGTGCCCATAATCATACAAAGCCCC-3′
Siliconized polypropylene 1.5 mL G-tube	Bio Plas	4167SLS50
Sodium dedecyl sulfate	Biosesang	S1010
Sodium deoxycholate	Sigma-Aldrich	D6750
SUPERase In Rnase inhibitor	Thermo Fisher Scientific	AM2694
SuperScript III reverse transcriptase	Thermo Fisher Scientific	18080093	Reverse transcriptase for library preparation
SuperScript IV reverse transcriptase	Thermo Fisher Scientific	18090010	Reverse transcriptase for qRT-PCR
SYBR gold nucleic acid gl stain	Thermo Fisher Scientific	S11494
T4 polynucleotide kinase	New England Biolabs	M0201S
T4 RNA ligase 1 (ssRNA Ligase)	New England Biolabs	M0204
T4 RNA ligase 2, truncated KQ	New England Biolabs	M0373
Thermomixer	Eppendorf ThermoMixer C with ThermoTop
Thymidine	Sigma-Aldrich	T9250
Tris-borate-EDTA buffer (TBE)	TaKara	T9122
Triton X-100	Promega	H5142
Ultralink Protein A sepharose beads	Thermo Fisher Scientific	22810	Protein A beads
Ultrasonicator	Bioruptor
Urea	Bio-basic	UB0148
Vortex mixer	DAIHAN Scientific	VM-10
Xylene cyanol	Sigma-Aldrich	X4126
γ-³²P-ATP (10 μCi/μL, 3.3 μM)	PerkinElmer	BLU502A100UC

Odniesienia

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