Sequence design
Nanostars have been designed utilizing NUPACK53 on the premise of printed in vitro outcomes11. For every design, ten NUPACK trials have been run, and the one which generated the bottom defect rating was chosen. Broccoli, Pepper, Mango and MS2 aptamer sequences have been taken from literature18,20,34,54. The wild-type KL (5′-GCGCGC) was tailored from the HIV-1 palindromic KL sequence32. Orthogonal KLs 5′-UCGCGA, 5′-GUCGAC and 5′-GGUACC have been taken from the research by Fabrini et al.12. KLs 5′-GUAUAC and 5′-UAUAUA have been designed by merely changing GC pairs with AU pairs. Non-palindromic KLs have been tailored from the 3sβ set designed by Stewart et al.11. Detailed design rules of nanostar stems and KLs might be present in Supplementary Part 1.1. All sequences are listed in Supplementary Desk 1.
RNA synthesis for in vitro characterization
All RNA strands for in vitro experiments have been transcribed from customized DNA templates synthesized by Built-in DNA Applied sciences as LabReady resuspensions with customary desalt purification. We annealed non-coding DNA templates with a 21-nt complement together with the T7 promoter area and a 4-nt sealing area (5′-GCGC). These templates have been annealed in 1× TE/50 mM NaCl from 90 °C to room temperature at −1 °C min−1 at 5 μM for storage and used at 0.01 μM throughout in vitro transcription. RNA strands have been transcribed in vitro at 37 °C utilizing 7.5% (v/v) T7 polymerase from the AmpliScribe T7-Flash transcription equipment (ASF3507, Biosearch Applied sciences), and transcription buffer ready in-house: 40 mM of Tris-HCl, 10 mM of NaCl, 30 mM MgCl2, 2 mM spermidine, 7.5 mM of every NTP and 10 mM DTT.
Plasmid improvement
Inserts have been instantly bought from Built-in DNA Applied sciences as two single-stranded, 5′-phosphorylated oligonucleotides containing the sequence of curiosity, flanked by NotI and SacII restriction websites. The 2 strands have been annealed in 50 mM NaCl and 1× TE buffer utilizing a warmth remedy protocol together with a 5-min soften at 90 °C, adopted by a sluggish temperature ramp at −1 °C min−1, and held at 20 °C. The ensuing merchandise have been double-stranded DNA fragments with sticky ends prepared for ligation. After annealing, strands have been purified with a DNA cleanup equipment (NEB, T1030). The DNA encoding the nanostar sequences was inserted within the pAV-U6+27-Twister-Broccoli (Addgene, 261587) plasmid. Plasmids have been ready by (1) digestion with NotI-HF (NEB, R3189S) (2 μl for 20-μl reactions) at 37 °C for 1 h, (2) purification with the DNA cleanup equipment, (3) digestion with SacII (NEB, R0157S) (2 μl for 20-μl reactions) at 37 °C for 1 h and (4) purification with a 0.8% 1× TAE agarose gel to pick out the product with the right measurement. Digested backbones have been lastly purified utilizing a gel extraction equipment (Qiagen, 28704). Digested spine and inserts have been ligated at a 1:10 molecular ratio by in a single day incubation with T4 DNA ligase (NEB, M0202S) at 4 °C. Ligated plasmids have been remodeled into 50 μl DF5Hα competent cells (Thermo Fisher, EC0112 and 18258012) following the producer’s protocol. We then extracted plasmid DNA utilizing a Miniprep equipment (Qiagen, 27106) following the producer’s protocol. Extracted plasmids have been lastly sequenced by Eurofins Genomics (entire plasmid sequencing service). The plasmid expressing MCP-mCherry was bought from Addgene (207668)55.
Cell tradition and upkeep
HEK293T (ATCC, CRL-3216), HeLa (ATCC, CCL-2) and U-2 OS (ATCC, HTB-96) cells have been grown in Dulbecco modified Eagle’s medium (DMEM), excessive glucose, pyruvate (Thermo Fisher, 11995065) containing 10% fetal bovine serum and 100 U ml−1 penicillin–streptomycin (Thermo Fisher) and maintained at 37 °C with 5% CO2 in a humidified incubator. Cells used for imaging have been cultured in µ-Slide 8-well excessive slides (Ibidi GmbH).
Transfection
Seeding density was tailored throughout cell varieties to realize ~70% confluence at transfection. Lipofectamine 2000 (Thermo Fisher, 11668019) was used for transfecting HEK293T cells. FuGene HD (Promega, E2311) was used for transfecting HeLa and U-2 OS cells because it demonstrated much less cytotoxicity as a consequence of transfection. For experiments involving the expression of a number of nanostars, the full quantity of plasmid DNA utilized in every experiment was stored fixed, with an equal proportion of every nanostar variant.
Complete RNA extraction
Cells have been transfected in 24-well plates, as described in Supplementary Part 1.5. We modified the medium 24 h after transfection, and picked up cells 48 h after transfection. For assortment, we aspirated media, washed with PBS and trypsinized the cells. After trypsinization, cells have been resuspended in PBS, lysed and RNA was purified utilizing the Monarch Complete RNA Miniprep Equipment (NEB, T2010S). RNA focus was estimated utilizing a Nanodrop 2000c by measuring absorption at 260 nm.
Dwell-cell staining
The tradition medium from in a single day incubation was aspirated and changed with recent medium supplemented with two drops of NucBlue Dwell reagent (Hoechst 33342 nuclear dye, Thermo Fisher, R37605) per millilitre of media, together with the suitable staining dyes in response to experimental circumstances. For circumstances involving the Broccoli aptamer, we used 40 µM of DFHBI (Lucerna; 400-5 mg). For experiments involving the Pepper aptamer, we provided 10 nM of HBC620 (MedChemExpress, HY-133520). Dwell cells have been then incubated for not less than 15 min at 37 °C earlier than imaging. Cells have been imaged within the presence of dyes.
Fastened cell staining and immunostaining
Mouse anti-coilin (Cajal physique colocalization) was bought from Abcam (ab11822; 1:1,900, 1 μg ml−1). Mouse anti-SC35 (nuclear speckle colocalization) was bought from Abcam (ab11826; 1:200, 5 μg ml−1). Mouse anti-fibrillarin (nucleolus colocalization) was bought from Antibodies.com (A85370; 1:200). Mouse anti-G3BP1 (stress granules colocalization) was bought from Thermo Fisher (66486-1-IG; 1:200, 5 μg ml−1). Mouse anti-DCP1A (P-body colocalization) was bought from Novus Organic (H00055802-M06; 1:200).
Earlier than fixation, cell tradition media have been eliminated and cells have been rinsed with PBS (Thermo Fisher, 10010023). Cells have been then mounted in a PBS buffer (Thermo Fisher, 14190144) containing 4% paraformaldehyde (Thermo Fisher, 043368.9M) for 10 min at room temperature, and washed with the PBS buffer thrice, every for five min. Subsequent, we permeabilized cells with 0.5% Triton X-100 (Sigma-Aldrich, 9002-93-1) in PBS buffer for 10 min and washed thrice. For imaging condensates involving the Mango aptamer, we added PBS supplemented with NucBlue reagent (Thermo Fisher, R37605) and 200 nM of TO1-B (ABM, G955). Cells have been incubated within the buffer for 15 min earlier than imaging. For experiments involving immunostaining, cells have been additional blocked utilizing 3% bovine serum albumin (BSA) (w/v; Sigma-Aldrich, 9048-46-8) in PBS buffer for 1 h, and washed thrice. Then, cells have been stained with corresponding main antibodies diluted to the above-mentioned concentrations with 3% BSA in PBS buffer and incubated at 4 °C in a single day. The following day, main antibodies have been eliminated and cells have been washed thrice earlier than the addition of secondary antibodies (Thermo Fisher, A-21236; 1:1,000 in 3% BSA in PBS buffer). We incubated cells in secondary antibodies for 1 h earlier than eradicating the buffer and washing them thrice with PBS. For the ultimate wash, PBS was supplemented with 40 μM DFHBI and NucBlue reagent. Cells have been incubated within the buffer for 15 min earlier than imaging.
Microscopy
FRAP and fusion experiments have been carried out with epifluorescence imaging utilizing a Nikon Eclipse TI-E inverted microscope and a 60× oil immersion goal. z-Stack confocal photos have been acquired utilizing a Nikon Ti microscope geared up with an NL5+ digital camera. Photographs in Fig. 4d,okay have been captured utilizing a Yokogawa CSU X1 spinning disk confocal on an inverted Zeiss stand. Hoechst (NucBlue staining) alerts have been detected within the UV channel (excitation 405 nm). Broccoli aptamer fluorescence was measured utilizing the GFP channel (excitation 488 nm). Mango aptamer fluorescence was measured utilizing the YFP channel (excitation 514 nm). Pepper aptamer, CY3 and mCherry fluorescence was detected utilizing the RFP channel (excitation 561 nm). Lastly, Alexa Fluor 647-labelled secondary antibody fluorescence was detected utilizing the 647 nm channel (excitation 647 nm).
Picture processing
To supply a extra complete view of condensate alerts throughout all planes, confocal micrographs within the manuscript figures are max-pixel-intensity z-projections, except in any other case specified within the determine caption. Detailed knowledge processing strategies and schematics might be present in Supplementary Info, together with condensate quantity and quantity quantification, nucleus quantity quantification, partition coefficient calculation for linked condensates (JR and JG), partition coefficient calculation for peptides and small-molecule dye, and the PCC and Manders’ overlap coefficient (M1 and M2) calculation.
FRAP
FRAP experiments have been carried out utilizing a Nikon Eclipse TI-E inverted microscope with a temperature management unit. In vitro samples have been loaded right into a house-made chamber and sealed with epoxy (Gorilla, 5-min set) for imaging. For in vivo experiments, cells have been stained and imaged within the Ibidi chamber described above. Condensates have been bleached with a 488-nm laser for 200 ms. For in vitro samples, imaging was captured as soon as earlier than bleaching and each 5 s for 10 min after bleaching. For in vivo samples, imaging was captured as soon as earlier than bleaching and each 200 ms for two min after bleaching or each 1.5 s for five min after bleaching. Photographs have been analysed by extracting time-dependent common intensities inside the bleached space and unbleached space. Information processing and becoming particulars are described in Supplementary Info.
Time-dependent coalescence evaluation
For in vitro experiments, RNA strands have been transcribed, labelled with 1% CY3-UTP, diluted ten occasions with transcription buffer and sealed in a chamber with epoxy, following the identical protocol as FRAP experiments. Samples have been imaged each 5 min for the primary 4 h, then each 20 min till 10 h. We monitored condensate fusion occasions utilizing a Nikon Eclipse TI-E inverted microscope with a temperature management unit. The temperature was maintained at 37 °C for all experiments.
For in vivo fusion experiments, we imaged cells (in media supplemented with 40 μM DFHBI and a couple of drops ml−1 NucBlue) each 5 min for 60 min below the confocal microscope. The temperature was maintained at 37 °C. Fusion occasions have been recognized manually. Information processing was carried out utilizing a script in Python3, as described in our earlier work11.
Circulation cytometry
Circulation cytometry experiments have been carried out utilizing a BD FACSAria circulate cytometer. Cells have been transfected in 24-well plates, as described in Supplementary Part 1.5. We modified the media 24 h after transfection, and picked up cells 48 h after transfection. For assortment, we aspirated media, washed with PBS and trypsinized the cells. After trypsinization, cells have been resuspended in PBS supplemented with 10% fetal bovine serum and dyes and filtered via a 40-μm cell strainer (Fisher Scientific, cat. no. 22363547) for circulate cytometry. Hoechst was detected utilizing a laser with Ex. 405 nm and a 450/50-nm filter; DFHBI was detected utilizing a laser with Ex. 488 nm and a 530/30-nm filter.
RT–qPCR
Reverse transcription was carried out with equal quantities of RNA utilizing the Protoscript II First Strand cDNA Synthesis Equipment and random hexamers (New England Biolabs). Reverse-transcription quantitative PCR (RT–qPCR) was then carried out utilizing tenfold diluted cDNA and the Luna Common qPCR Grasp Combine (New England Biolabs) within the CFX Actual-Time PCR system (Bio-Rad), courtesy of the UCLA Virology Core. The qPCR circumstances used have been as beforehand described56,57. Goal transcript ranges have been decided by normalizing the cycle threshold worth of the goal transcript to that of the housekeeping gene RPS11 transcript. Fold change was calculated utilizing this normalized worth relative to Lipofectamine management expression ranges. For RT–qPCR primers, see Supplementary Desk 4.
Polyacrylamide gel electrophoresis
Gel pre-mix was ready by including 42 g of urea to nanopure water, the combination was then heated till the urea utterly dissolved. This combination was allowed to chill to room temperature, after which a 40% (v/v) 19:1 acrylamide:bis-acrylamide answer was added within the applicable quantity for the specified proportion (last quantity of 100 ml). To begin polymerization, 8 ml of pre-mix was added in applicable ratios with TBE and nanopure water, ammonium persulfate and tetramethylethylenediamine. Gels have been forged in 8 cm × 8 cm, 1-mm-thick disposable mini gel cassettes (Thermo Scientific, NC2010) and allowed to polymerize for 30 min earlier than electrophoresis. After curing, the gel was pre-run in a 1× TBE buffer for 30 min. Wells have been washed rigorously to take away extreme urea. Samples and a low-range ssRNA ladder (NEB, N0364S) have been ready by mixing particular person strands with denaturing RNA loading dye (NEB, B0363S), then heated at 70 °C for 10 min and instantly positioned on ice. Owing to the low expression of exogenous RNA in mammalian cells, 5 μg of complete RNA extraction was loaded into every effectively. Gels have been run at room temperature at 100 V in 1× TBE except in any other case famous. After electrophoresis, the gels have been washed thrice, every for five min, with nanopure water, then stained with DFHBI-1T staining buffer (10 μM DFHBI-1T, 40 mM HEPES, 100 mM KCl and 1 mM MgCl2) for 15 min. After staining, gels have been imaged utilizing the Bio-Rad Gel Imaging Techniques. Then, gels have been washed thrice, every for five min, to take away the DFHBI-1T and stained in 1× SYBR Gold Nucleic Acid Gel Stain for 15 min and imaged once more.
Statistics and reproducibility
At the very least three unbiased organic replicates have been examined for every situation. For microscopy imaging, not less than three totally different fields of view have been captured for every replicate. No knowledge have been excluded from the analyses.