Name: investigation of protein recruitment to dna lesions using 405 nm laser micro-irradiation
Uploaded: 2018-03-20T15:00:00
Description: Watch this Scientific Journal Video about Investigation of Protein Recruitment to DNA Lesions Using 405 Nm Laser Micro-irradiation at JoVE.com

This work was supported by the Natural Sciences and Engineering Research Council of Canada [Discovery grant 5026 to A.M] and by a Next-Generation of Scientists Scholarship from the Cancer Research Society [21531 to A.M]. We thank Jean-Fran&#231;ois Lucier for providing excellent quality control of the Fiji Python scripts and advice on statistical analysis. We thank Dr. Stephanie A. Yazinski for the IF fixation solution recipe. We thank Paul-Ludovic Karsenti for help with laser power measurements.

1. Pre-sensitization of Cells
<ol>
	<li>24 h prior to the micro-irradiation experiment, seed 40,000 U2OS cells per well in 1x DMEM containing 10% FBS in 8-well culture slides with 170 &#181;m-thick coverslip-like glass/polymer bottoms to ensure maximal transmittance of 405 nm laser light and excellent imaging with a laser-scanning inverted confocal microscope. If using an 8-well microslide, use 500 &#181;L of media or solutions per well for all subsequent treatments and wash steps of the protocol. 
	NOTE: Due to t...

<ol>
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Using the methods outlined above, 405 nm laser micro-irradiation of cells pre-sensitized with BBET or BrdU allows the localized generation of DNA lesions including DSBs within the nuclei of adherent human cells. Kinetics of DDR at these DSBs are similar to those generated with other methods in eukaryotic cells9,18,19. DSB resection at micro-irradiated sites leads to ssDNA-generation which can be followed using a RPA32-targeting ...

Cells are constantly exposed to endogenous and exogenous sources of DNA damage that threaten their genomic integrity. The DDR is an ensemble of signaling pathways that detect, signal, and repair DNA lesions to sustain genome stability. At DNA double-stranded breaks (DSBs), the DDR occurs mainly on two complementary platforms: &#947;-H2A.X-labeled chromatin and a resected single-stranded DNA (ssDNA) region typically coated with the ssDNA-binding complex RPA1,2.
UV-laser micro-irradiation of cells pre-sensitized with the thymidine analogue 5-bromo-2&#39;deoxyuridine (BrdU) or the bisbenzimide ethoxide trihydrochloride (BBET, Hoechst 33342) DNA dye creates a mixture of DNA lesions including single-stranded breaks (SSBs) and DSBs which elicit a localized DDR on both the chromatin and ssDNA platforms3,4. Previous work showed that recruitment of genome maintenance factors to these two distinct platforms at DSB can be discriminated using high energy UV-A lasers (335-365 nm) combined with IF2,5. Microscopes equipped with such lasers are costly as they require a high energy laser and dedicated UV-A transmitting objectives making them far less prevalent in academic and pharmaceutical settings than laser-scanning confocal microscopes with 405 nm laser lines. The study of protein recruitment and exchange at micro-irradiated sites is also precluded by the laborious manual image analysis required to describe the dynamic behavior of genome maintenance factors.
Here, we show that the pre-sensitization of cells with BrdU or BBET nucleic acid stain followed by micro-irradiation using a 405 nm laser on a common confocal microscope allows the monitoring of genome maintenance factor dynamics at DNA lesions. Using &#947;-H2A.X or RPA complex subunits as platform markers together with z-stacking for greater depth of field and deconvolution for improved resolution allows the experimenter to discriminate factors that are locally recruited to DSBs from those that spread to large chromatin domains surrounding the initial lesion. This sub-classification according to distinct intra-nuclear compartments helps refine the potential roles of uncharacterized proteins recruited to micro-irradiated sites. Moreover, we provide convenient protocols and optimized pipelines to rapidly analyze the dynamics of genome maintenance factors using the open-source software Fiji (an ImageJ distribution)6,7,8. These refinements to current micro-irradiation methods render the study of the DDR possible in virtually any laboratory setting.

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	<tbody>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Olympus FLUOVIEW FV3000 resonant laser scanning confocal microscope</td>
			<td style="width:167px;">Olympus</td>
			<td style="width:171px;"></td>
			<td style="width:179px;"></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">FluoView FV3000 software (version 2.1)</td>
			<td>Olympus</td>
			<td></td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">405 nm laser</td>
			<td>Coherent</td>
			<td></td>
			<td>Radiation source</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Microscope incubator AIO-UNO-OLYUS-1</td>
			<td>Okolab</td>
			<td>OKO-UNO-1</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">60X /1.4 Objective</td>
			<td>Olympus</td>
			<td></td>
			<td>Oil immersion objective</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">8-well culture slides on coverglass (X-well)</td>
			<td>Sarstedt</td>
			<td>94.6190.802</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">U2OS osteosarcoma human cell line</td>
			<td>ATCC</td>
			<td>HTB-96</td>
			<td>Stable cell lines&#160;</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">4&#8217;,6-Diamidino-2-Phenylindole (DAPI)</td>
			<td>ThermoFisher</td>
			<td>D1306</td>
			<td>Caution toxic</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">5-bromo-2&#8242;-deoxyuridine&#160;(BrdU)&#160;</td>
			<td>Sigma-Aldrich</td>
			<td>59-14-3</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Paraformaldehyde</td>
			<td>Sigma-Aldrich</td>
			<td>30525-89-4</td>
			<td>Caution toxic</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Bisbenzimide H 33342 (Hoechst 33342)</td>
			<td>ThermoFisher</td>
			<td>62249</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Bovine serum albumin (BSA)</td>
			<td>ThermoFisher</td>
			<td>BP1600-100</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Trypsin EDTA 0.1%&#160;</td>
			<td>ThermoFisher</td>
			<td>15400-054</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Triton X-100&#160;</td>
			<td>BioShop</td>
			<td>TRX777.100</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Tween-20&#160;</td>
			<td>ThermoFisher</td>
			<td>BP337-500</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Sucrose&#160;</td>
			<td>BioShop</td>
			<td>SUC507</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">JetPRIME transfection reagent&#160;</td>
			<td>Polyplus</td>
			<td>114-07</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">ProLong Diamond Antifade mountant with DAPI&#160;</td>
			<td>ThermoFisher</td>
			<td>P36962</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">DMEM 1X, + phenol red</td>
			<td>Wisent&#160;</td>
			<td>319-005-CL</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">DMEM 1X, - phenol red</td>
			<td>Wisent</td>
			<td>319-051-CL</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Fetal bovine serum (FBS)</td>
			<td>Wisent&#160;</td>
			<td>080-150</td>
			<td></td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Mouse anti-RPA32 antibody</td>
			<td>Abcam</td>
			<td>ab2175</td>
			<td>1:500 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Rabbit anti-&#947;-H2A.X antibody</td>
			<td>Cell Signaling&#160;</td>
			<td>9718S</td>
			<td>1:500 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Rabbit Anti-53BP1 antibody</td>
			<td>Cell Signaling&#160;</td>
			<td>4937S</td>
			<td>1:500 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Rabbit Anti-PRP19 antibody</td>
			<td>Abcam</td>
			<td>ab27692</td>
			<td>1:500 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Goat anti-rabbit IgG Alexa Fluor 647</td>
			<td>Cell Signaling&#160;</td>
			<td>4414S</td>
			<td>1:250 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Goat anti-mouse&#160; IgG Alexa Fluor 488&#160;</td>
			<td>Cell Signaling&#160;</td>
			<td>4408S</td>
			<td>1:250 for IF</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">Fiji image analysis open-source software&#160;</td>
			<td></td>
			<td></td>
			<td>https://fiji.sc</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:508px;">1918-K Power meter&#160; with a 918D-SL-0D3 sensor</td>
			<td>Newport</td>
			<td></td>
			<td></td>
		</tr>
	</tbody>
</table>

investigation of protein recruitment to dna lesions using 405 nm laser micro-irradiation

The DNA Damage Response (DDR) uses a plethora of proteins to detect, signal, and repair DNA lesions. Delineating this response is critical to understand genome maintenance mechanisms. Since recruitment and exchange of proteins at lesions are highly dynamic, their study requires the ability to generate DNA damage in a rapid and spatially-delimited manner. Here, we describe procedures to locally induce DNA damage in human cells using a commonly available laser-scanning confocal microscope equipped with a 405 nm laser line. Accumulation of genome maintenance factors at laser stripes can be assessed by immunofluorescence (IF) or in real-time using proteins tagged with fluorescent reporters. Using phosphorylated histone H2A.X (&#947;-H2A.X) and Replication Protein A (RPA) as markers, the method provides sufficient resolution to discriminate locally-recruited factors from those that spread on adjacent chromatin. We further provide ImageJ-based scripts to efficiently monitor the kinetics of protein relocalization at DNA damage sites. These refinements greatly simplify the study of the DDR dynamics.

Following micro-irradiation, cells are allowed to recover for a specific period of time depending on the nature of the genome maintenance proteins1,12. DSBs will be processed by nucleases, most extensively during the S and G2 phases of the cell cycle, to create a limited region of ssDNA which is rapidly coated by RPA and other genome maintenance factors9. This ssDNA region is surrounded by chromatin which i...

Watch this Scientific Journal Video about Investigation of Protein Recruitment to DNA Lesions Using 405 Nm Laser Micro-irradiation at JoVE.com

Investigation of Protein Recruitment to DNA Lesions Using 405 Nm Laser Micro-irradiation

Studying DNA damage repair kinetics requires a system to induce lesions at defined sub-nuclear regions. We describe a method to create localized double-stranded breaks using a laser-scanning confocal microscope equipped with a 405 nm laser and provide automated procedures to quantify the dynamics of repair factors at these lesions.

The DNA Damage Response (DDR) uses a plethora of proteins to detect, signal, and repair DNA lesions. Delineating this response is critical to understand ...

The overall goal of this procedure is to create localized DNA double-stranded breaks using a broadly available 405 nanometer laser scanning confocal microscope, and provide automated procedures to quantify the dynamics of DNA repair factors at these lesions. This method can be used to determine whether a given protein is recruited to double-stranded DNA breaks, and delineate the signaling pathways that regulate its accumulation at DNA lesions. The technique uses a commonly available confocal microscope system to locally induce DNA damage.This allows virtually any laboratory to study the kinetics of the DNA damage response. If monitoring the live recruitment of a fluorescently-labeled protein, perform transient transfection, or selection of stable cell lines expressing the protein of interest, fused to a fluorescent reporter. 24 hours prior to the micro-irradiation experiment, seed 40, 000 U2OS cells per well in DMEM 1X containing 10%FBS, in eight-well culture slides, with 170 micron thick coverslip-like glass polymer bottoms.Incubate the cells overnight at 37 degrees Celsius, with 5%CO2. To increase the number of double-stranded breaks generated by exposure to the 405 nanometer laser, add BBET to the cells, at 10 micrograms per milliliter in the appropriate medium. Treat the cells for 15 minutes in a cell culture incubator at 37 degrees Celsius.Prior to micro-irradiation, use a micropipette to rinse the cells twice with medium without phenol red, to ensure maximal exposure of the cells to the 405 nanometer laser. Any confocal microscope equipped with the 405 nanometer laser can be used for this method. Users need to carefully calibrate their system to achieve physiological levels of DNA damage.We describe how to do this in the detailed protocol. Select a suitable laser scanning confocal microscope equipped with a 405 nanometer laser. Turn on the microscope and the environmental chamber.Select fields with well-distributed cells, adjust the focus, and register their position to facilitate image acquisition after the immunofluorescence protocol. If using a fluorescently-labeled protein for live imaging, acquire at least one image that will serve as a pre-damage reference point, to monitor the kinetics of protein recruitment after micro-irradiation. For immunofluorescence experiments using BBET-labeled cells adjust the focus on the cells using the 405 nanometer laser at the lowest laser power sufficient to visualize the cells, to avoid unwarranted DNA damage.If using cells expressing the fluorescently-labeled protein of interest, select a focal plane with representative fluorescence intensity. Configure the microscope for the micro-irradiation step using the fluorescence-recovery after photobleaching module of the system. Using the FRAP module of the microscope system, select regions of interest that will be micro-irradiated.Once this is done, micro-irradiate the cells. Typically, chromatin-associated factors will be recruited to double-stranded breaks within two minutes. Resection of the breaks by nucleases will generate single-stranded DNA, and promote the recruitment of homologous recombination factors which become detectable 10 minutes after micro-irradiation.After micro-irradiation, place the multi-well slides back into the incubator at 37 degrees Celsius with 5%CO2 for the required duration prior to processing samples for immunofluorescence. Or, proceed immediately with live time-lapse imaging as detailed in the text protocol. To begin analysis, open the acquired images in Fiji.Select the Damage Analyzer from the pull-down plug-ins menu in the micro-irradiation analysis suite. Define the time units and the time interval between frames, then register the image series using the StackReg algorithm. Follow the prompts to define a background region of interest, or ROI, in each micro-irradiated cell.Also, define non-irradiated and irradiated ROIs in each micro-irradiated cell. Once all ROI data have been collected over the full time-lapse series, save the file created by the plug-in containing the results as a comma-delimited file. This file contains measurements of the mean intensity for each time point and each ROI.Perform the analysis using the plug-in for all micro-irradiated cells, and graph the relative enrichment at micro-irradiated regions over time. This step should be repeated for at least 15 to 30 cells, and the mean enrichment and the standard errors of the mean for each data point should be calculated and plotted. Using a micropipette, carefully remove the media from the wells of the multi-well microscopy slides.Immediately wash the cells with 500 microliters of IF washing solution by changing the solution twice without waiting. Then, incubate on ice for five minutes, with 500 microliters of ice-cold IF pre-and post-extraction solution. Swirl gently by hand for 15 to 30 seconds to perform the pre-extraction step that removes most cytoplasmic and nucleoplasmic proteins, and maximizes the signal from chromatin and DNA associated factors.Next, wash the cells twice with 500 microliters of IF washing solution. Then, add 500 microliters of IF fixation solution, and incubate for 15 minutes at room temperature. After washing twice with 500 microliters of IF washing solution, incubate on ice for five minutes in 500 microliters of ice-cold IF pre-and post-extraction solution.Swirl the slide gently by hand to perform the permeabilization step. Wash the cells twice with 500 microliters of IF washing solution. Then, incubate at least 30 minutes at room temperature with 500 microliters of IF blocking solution.Remove the blocking solution using a micropipette and add 250 microliters of primary antibody solution. Then, incubate the cells overnight in a humidified chamber at 4 degrees Celsius. The next day, wash the cells four times for five minutes in 500 microliters of IF washing solution with gentle agitation.Then, incubate the cells for one hour at 37 degrees Celsius with 250 microliters of secondary antibodies diluted in blocking solution in a humidified chamber. Protect the samples from light upon addition of fluorescently-labeled secondary antibodies. Then, wash the cells four times each for five minutes in a 500 microliters of IF washing solution with gentle agitation.Incubate the cells at room temperature for five minutes in 500 microliters of 1X PBS, containing one microgram per milliliter of DAPI to stain the nuclei. After washing the cells twice with 500 microliters of 1X PBS, leave cells in 500 microliters of 1X PBS solution for imaging. Using gridded slides or registered stage positions, find the micro-irradiated cells using a well-characterized DNA damage marker.Image the multi-well culture slides in all relevant channels using the appropriate settings on a laser scanning confocal microscope. Laser micro-irradiation of pre-sensitized cells leads to the production of DNA double-stranded breaks, which are resected by nucleases to generate single-stranded DNA. Proteins or modifications that spread to large chromatin domains appear as broad stripes within two minutes of micro-irradiation.This is exemplified by the pattern observed with antibodies targeting the phosphorylated histone variant H2A. X.The single-stranded DNA can be visualized at later time points as punctate foci using antibodies against replication protein A.Using this method, it is evident that 53BP1 is recruited onto large chromatin domains, whereas the PRP19 E3 ubiquitin ligase is recruited onto RPA-coded single-stranded DNA. Transfection of plasmids encoding proteins tagged with fluorescent reporters, followed by micro-irradiation, allows the monitoring of protein recruitment to DNA lesions in real time.Micro-irradiation of BRDU pre-sensitized cells transfected with plasmids expressing EGFP, or RPA32 fused to GFP, show that RPA32-GFP but not EGFP alone, is rapidly recruited to the single-stranded DNA created by resection of the double-stranded DNA breaks. This graph shows the quantification of the RPA32 GFP signal enrichment over time at micro-irradiated loci from 15 independent cells analyzed with the micro-irradiation analysis Fiji plug-in. Once mastered, this technique can be done in approximately four hours for live imaging of 10 to 15 individual cells expressing fluorescently-labeled proteins, and within two days when immunofluorescence is used to monitor protein recruitment at micro-irradiated loci.After watching this video, you should have a good understanding of how to configure a laser scanning microscope and use it to micro-irradiate cells and monitor the recruitment of DNA repair factors to sites of damage, both in real time and in fixed cells. While attempting this procedure, it's important to remember that the conditions described here generate double-stranded breaks, but also other types of lesions. But the user can alter micro-irradiation and pre-sensitization methods to create specific types of lesions relevant to their research.Following this procedure, depletion of established DNA damage response factors are mutation of specific domains in the protein of interest can be performed to provide additional insight into the recruitment mechanism of these factors at DNA breaks. Don't forget that working with lasers and paraformaldehyde can be extremely hazardous, and precautions such as wearing personal protection equipment, and working in a chemical hood when required should always be taken while performing this procedure.

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Research

JoVE Journal

Genetics

RNA Interference-based Investigation of the Function of Heat Shock Protein 27 during Corneal Epithelial Wound Healing

Small interfering RNA (siRNA) is among the most widely used RNA interference methods for the short-term silencing of protein-coding genes. siRNA is a synthetic RNA duplex created to specifically target a mRNA transcript to induce its degradation and it has been used to identify novel pathways in various cellular processes. Few reports exist regarding the role of phosphorylated heat shock protein 27 (HSP27) in corneal epithelial wound healing. Herein, cultured human corneal epithelial cells were divided into a scrambled control-siRNA transfected group and a HSP27-specific siRNA-transfected group. Scratch-induced directional wounding assays, and western blotting, and flow cytometry were then performed. We conclude that HSP27 has roles in corneal epithelial wound healing that may involve epithelial cell apoptosis and migration. Here, step-by-step descriptions of sample preparation and the study protocol are provided.

Herein, we present a protocol to use heat shock protein 27 (HSP27)-specific small interfering RNA to assess the function of HSP27 during corneal epithelial wound healing. RNA interference is the best method for effectively knocking-down gene expression to investigate protein function in various cell types.

Small interfering RNA (siRNA) is among the most widely used RNA interference methods for the short-term silencing of protein-coding genes. siRNA is a ...

Tools to Study the Role of Architectural Protein HMGB1 in the Processing of Helix Distorting, Site-specific DNA Interstrand Crosslinks

High mobility group box 1 (HMGB1) protein is a non-histone architectural protein that is involved in regulating many important functions in the genome, such as transcription, DNA replication, and DNA repair. HMGB1 binds to structurally distorted DNA with higher affinity than to canonical B-DNA. For example, we found that HMGB1 binds to DNA interstrand crosslinks (ICLs), which covalently link the two strands of the DNA, cause distortion of the helix, and if left unrepaired can cause cell death. Due to their cytotoxic potential, several ICL-inducing agents are currently used as chemotherapeutic agents in the clinic. While ICL-forming agents show preferences for certain base sequences (e.g., 5&#39;-TA-3&#39; is the preferred crosslinking site for psoralen), they largely induce DNA damage in an indiscriminate fashion. However, by covalently coupling the ICL-inducing agent to a triplex-forming oligonucleotide (TFO), which binds to DNA in a sequence-specific manner, targeted DNA damage can be achieved. Here, we use a TFO covalently conjugated on the 5&#39; end to a 4&#39;-hydroxymethyl-4,5&#39;,8-trimethylpsoralen (HMT) psoralen to generate a site-specific ICL on a mutation-reporter plasmid to use as a tool to study the architectural modification, processing, and repair of complex DNA lesions by HMGB1 in human cells. We describe experimental techniques to prepare TFO-directed ICLs on reporter plasmids, and to interrogate the association of HMGB1 with the TFO-directed ICLs in a cellular context using chromatin immunoprecipitation assays. In addition, we describe DNA supercoiling assays to assess specific architectural modification of the damaged DNA by measuring the amount of superhelical turns introduced on the psoralen-crosslinked plasmid by HMGB1. These techniques can be used to study the roles of other proteins involved in the processing and repair of TFO-directed ICLs or other targeted DNA damage in any cell line of interest.

Targeted DNA damage can be achieved by tethering a DNA damaging agent to a triplex-forming oligonucleotide (TFO). Using modified TFOs, DNA damage-specific protein association, and DNA topology modification can be studied in human cells by the utilization of modified chromatin immunoprecipitation assays and DNA supercoiling assays described herein.

High mobility group box 1 (HMGB1) protein is a non-histone architectural protein that is involved in regulating many important functions in the genome, ...

Protocols for C-Brick DNA Standard Assembly Using Cpf1

CRISPR-associated protein Cpf1 cleaves double-stranded DNA under the guidance of CRISPR RNA (crRNA), generating sticky ends. Because of this characteristic, Cpf1 has been used for the establishment of a DNA assembly standard called C-Brick, which has the advantage of long recognition sites and short scars. On a standard C-Brick vector, there are four Cpf1 recognition sites &#8211; the prefix (T1 and T2 sites) and the suffix (T3 and T4 sites) &#8211; flanking biological DNA parts. The cleavage of T2 and T3 sites produces complementary sticky ends, which allow for the assembly of DNA parts with T2 and T3 sites. Meanwhile, a short &#34;GGATCC&#34; scar is generated between parts after assembly. As the newly formed plasmid once again contains the four Cpf1 cleavage sites, the method allows for the iterative assembly of DNA parts, which is similar to those of BioBrick and BglBrick standards. A procedure outlining the use of the C-Brick standard to assemble DNA parts is described here. The C-Brick standard can be widely used by scientists, graduate and undergraduate students, and even amateurs.

CRISPR-associated protein Cpf1 can be guided by a specially designed CRISPR RNA (crRNA) to cleave double-stranded DNA at desired sites, generating sticky ends. Based on this characteristic, a DNA assembly standard (C-Brick) was established, and a protocol detailing its use is described here.

CRISPR-associated protein Cpf1 cleaves double-stranded DNA under the guidance of CRISPR RNA (crRNA), generating sticky ends. Because of this ...

Genome-wide Mapping of Protein-DNA Interactions with ChEC-seq in Saccharomyces cerevisiae

Genome-wide mapping of protein-DNA interactions is critical for understanding gene regulation, chromatin remodeling, and other chromatin-resident processes. Formaldehyde crosslinking followed by chromatin immunoprecipitation and high-throughput sequencing (X-ChIP-seq) has been used to gain many valuable insights into genome biology. However, X-ChIP-seq has notable limitations linked to crosslinking and sonication. Native ChIP avoids these drawbacks by omitting crosslinking, but often results in poor recovery of chromatin-bound proteins. In addition, all ChIP-based methods are subject to antibody quality considerations. Enzymatic methods for mapping protein-DNA interactions, which involve fusion of a protein of interest to a DNA-modifying enzyme, have also been used to map protein-DNA interactions. We recently combined one such method, chromatin endogenous cleavage (ChEC), with high-throughput sequencing as ChEC-seq. ChEC-seq relies on fusion of a chromatin-associated protein of interest to micrococcal nuclease (MNase) to generate targeted DNA cleavage in the presence of calcium in living cells. ChEC-seq is not based on immunoprecipitation and so circumvents potential concerns with crosslinking, sonication, chromatin solubilization, and antibody quality while providing high resolution mapping with minimal background signal. We envision that ChEC-seq will be a powerful counterpart to ChIP, providing an independent means by which to both validate ChIP-seq findings and discover new insights into genomic regulation.

Genome-wide Mapping of Protein-DNA Interactions with ChEC-seq in Saccharomyces cerevisiae

We describe chromatin endogenous cleavage coupled with high-throughput sequencing (ChEC-seq), a chromatin immunoprecipitation (ChIP)-orthogonal method for mapping protein binding sites genome-wide with micrococcal nuclease (MNase) fusion proteins.

Genome-wide mapping of protein-DNA interactions is critical for understanding gene regulation, chromatin remodeling, and other chromatin-resident ...

Laser Microirradiation to Study In Vivo Cellular Responses to Simple and Complex DNA Damage

DNA damage induces specific signaling and repair responses in the cell, which is critical for protection of genome integrity. Laser microirradiation became a valuable experimental tool to investigate the DNA damage response (DDR) in vivo. It allows real-time high-resolution single-cell analysis of macromolecular dynamics in response to laser-induced damage confined to a submicrometer region in the cell nucleus. However, various laser conditions have been used without appreciation of differences in the types of damage induced. As a result, the nature of the damage is often not well characterized or controlled, causing apparent inconsistencies in the recruitment or modification profiles. We demonstrated that different irradiation conditions (i.e., different wavelengths as well as different input powers (irradiances) of a femtosecond (fs) near-infrared (NIR) laser) induced distinct DDR and repair protein assemblies. This reflects the type of DNA damage produced. This protocol describes how titration of laser input power allows induction of different amounts and complexities of DNA damage, which can easily be monitored by detection of base and crosslinking damages, differential poly (ADP-ribose) (PAR) signaling, and pathway-specific repair factor assemblies at damage sites. Once the damage conditions are determined, it is possible to investigate the effects of different damage complexity and differential damage signaling as well as depletion of upstream factor(s) on any factor of interest.

Laser Microirradiation to Study In Vivo Cellular Responses to Simple and Complex DNA Damage

The goal of this protocol is to describe how to use laser microirradiation to induce different types of DNA damage, including relatively simple strand breaks and complex damage, to study DNA damage signaling and repair factor assembly at damage sites in vivo.

DNA damage induces specific signaling and repair responses in the cell, which is critical for protection of genome integrity. Laser microirradiation ...

Investigation of RNA Synthesis Using 5-Bromouridine Labelling and Immunoprecipitation

When steady state RNA levels are compared between two conditions, it is not possible to distinguish whether changes are caused by alterations in production or degradation of RNA. This protocol describes a method for measurement of RNA production, using 5-Bromouridine labelling of RNA followed by immunoprecipitation, which enables investigation of RNA synthesized within a short timeframe (e.g., 1 h). The advantage of 5-Bromouridine-labelling and immunoprecipitation over the use of toxic transcriptional inhibitors, such as &#945;-amanitin and actinomycin D, is that there are no or very low effects on cell viability during short-term use. However, because 5-Bromouridine-immunoprecipitation only captures RNA produced within the short labelling time, slowly produced as well as rapidly degraded RNA can be difficult to measure by this method. The 5-Bromouridine-labelled RNA captured by 5-Bromouridine-immunoprecipitation can be analyzed by reverse transcription, quantitative polymerase chain reaction, and next generation sequencing. All types of RNA can be investigated, and the method is not limited to measuring mRNA as is presented in this example.

This method can be used to measure RNA synthesis. 5-Bromouridine is added to cells and incorporated into synthesized RNA. RNA synthesis is measured by RNA extraction immediately after labelling, followed by 5-Bromouridine-targeted immunoprecipitation of labelled RNA and analysis by reverse transcription and quantitative polymerase chain reaction.

When steady state RNA levels are compared between two conditions, it is not possible to distinguish whether changes are caused by alterations in ...

A Simple, Rapid, and Quantitative Assay to Measure Repair of DNA-protein Crosslinks on Plasmids Transfected into Mammalian Cells

The purpose of this method is to provide a flexible, rapid, and quantitative technique to examine the kinetics of DNA-protein crosslink (DPC) repair in mammalian cell lines. Rather than globally assaying removal of xenobiotic-induced or spontaneous chromosomal DPC removal, this assay examines the repair of a homogeneous, chemically defined lesion specifically introduced at one site within a plasmid DNA substrate. Importantly, this approach avoids the use of radioactive materials and is not dependent on expensive or highly-specialized technology. Instead, it relies on standard recombinant DNA procedures and widely available real-time, quantitative polymerase chain reaction (qPCR) instrumentation. Given the inherent flexibility of the strategy utilized, the size of the crosslinked protein, as well as the nature of the chemical linkage and the precise DNA sequence context of the attachment site can be varied to address the respective contributions of these parameters to the overall efficiency of DPC repair. Using this method, plasmids containing a site-specific DPC were transfected into cells and low molecular weight DNA recovered at various times post-transfection. Recovered DNA is then subjected to strand-specific primer extension (SSPE) using a primer complementary to the damaged strand of the plasmid. Since the DPC lesion blocks Taq DNA polymerase, the ratio of repaired to un-repaired DNA can be quantitatively assessed using qPCR. Cycle threshold (CT) values are used to calculate percent repair at various time points in the respective cell lines. This SSPE-qPCR method can also be used to quantitatively assess the repair kinetics of any DNA adduct that blocks Taq polymerase.

The goal of this protocol is to quantify the repair of defined DNA-protein crosslinks on plasmid DNA. Lesioned plasmids are transfected into recipient mammalian cell lines and low-molecular weight harvested at multiple time points post-transfection. DNA repair kinetics are quantified using strand-specific primer extension followed by qPCR.

The purpose of this method is to provide a flexible, rapid, and quantitative technique to examine the kinetics of DNA-protein crosslink (DPC) repair in ...

Rare Event Detection Using Error-corrected DNA and RNA Sequencing

Conventional next-generation sequencing techniques (NGS) have allowed for immense genomic characterization for over a decade. Specifically, NGS has been used to analyze the spectrum of clonal mutations in malignancy. Though far more efficient than traditional Sanger methods, NGS struggles with identifying rare clonal and subclonal mutations due to its high error rate of ~0.5&#8211;2.0%. Thus, standard NGS has a limit of detection for mutations that are &#62;0.02 variant allele fraction (VAF). While the clinical significance for mutations this rare in patients without known disease remains unclear, patients treated for leukemia have significantly improved outcomes when residual disease is &#60;0.0001 by flow cytometry. In order to mitigate this artefactual background of NGS, numerous methods have been developed. Here we describe a method for Error-corrected DNA and RNA Sequencing (ECS), which involves tagging individual molecules with both a 16 bp random index for error-correction and an 8 bp patient-specific index for multiplexing. Our method can detect and track clonal mutations at variant allele fractions (VAFs) two orders of magnitude lower than the detection limit of NGS and as rare as 0.0001 VAF.

Next-generation sequencing (NGS) is a powerful tool for genomic characterization that is limited by the high error rate of the platform (~0.5&#8211;2.0%). We describe our methods of error-corrected sequencing that allow us to obviate the NGS error rate and detect mutations at variant allele fractions as rare as 0.0001.

Conventional next-generation sequencing techniques (NGS) have allowed for immense genomic characterization for over a decade. Specifically, NGS has been ...

Mass Spectrometry-Based Proteomics Analyses Using the OpenProt Database to Unveil Novel Proteins Translated from Non-Canonical Open Reading Frames

Genome annotation is central to today's proteomic research as it draws the outlines of the proteomic landscape. Traditional models of open reading frame (ORF) annotation impose two arbitrary criteria: a minimum length of 100 codons and a single ORF per transcript. However, a growing number of studies report expression of proteins from allegedly non-coding regions, challenging the accuracy of current genome annotations. These novel proteins were found encoded either within non-coding RNAs, 5' or 3' untranslated regions (UTRs) of mRNAs, or overlapping a known coding sequence (CDS) in an alternative ORF. OpenProt is the first database that enforces a polycistronic model for eukaryotic genomes, allowing annotation of multiple ORFs per transcript. OpenProt is freely accessible and offers custom downloads of protein sequences across 10 species. Using OpenProt database for proteomic experiments enables novel proteins discovery and highlights the polycistronic nature of eukaryotic genes. The size of OpenProt database (all predicted proteins) is substantial and need be taken in account for the analysis. However, with appropriate false discovery rate (FDR) settings or the use of a restricted OpenProt database, users will gain a more realistic view of the proteomic landscape. Overall, OpenProt is a freely available tool that will foster proteomic discoveries.

OpenProt is a freely accessible database that enforces a polycistronic model of eukaryotic genomes. Here, we present a protocol for the use of OpenProt databases when interrogating mass spectrometry datasets. Using OpenProt database for analysis of proteomic experiments allows for discovery of novel and previously undetectable proteins.

Genome annotation is central to today's proteomic research as it draws the outlines of the proteomic landscape. Traditional models of open reading frame ...

In Vitro Biochemical Assays using Biotin Labels to Study Protein-Nucleic Acid Interactions

Protein-nucleic acid interactions play important roles in biological processes such as transcription, recombination, and RNA metabolism. Experimental methods to study protein-nucleic acid interactions require the use of fluorescent tags, radioactive isotopes, or other labels to detect and analyze specific target molecules. Biotin, a non-radioactive nucleic acid label, is commonly used in electrophoretic mobility shift assays (EMSA) but has not been regularly employed to monitor protein activity during nucleic acid processes. This protocol illustrates the utility of biotin labeling during in vitro enzymatic reactions, demonstrating that this label works well with a range of different biochemical assays. Specifically, in alignment with previous findings using radioisotope 32P-labeled substrates, it is confirmed via biotin-labeled EMSA that MEIOB (a protein specifically involved in the meiotic recombination) is a DNA-binding protein, that MOV10 (an RNA helicase) resolves biotin-labeled RNA duplex structures, and that MEIOB cleaves biotin-labeled single-stranded DNA. This study demonstrates that biotin is capable of substituting 32P in various nucleic acid-related biochemical assays in vitro.&#160;

Presented here are protocols for in vitro biochemical assays using biotin labels that may be widely&#160;applicable for studying protein-nucleic acid interactions.

Protein-nucleic acid interactions play important roles in biological processes such as transcription, recombination, and RNA metabolism. Experimental ...