membrane-targeted fluorophores
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** I have used membrane-targeted fluorophores for visualizing neuronal morphology off and on over the years. Some colleagues have warned me about their potential side affects, and although I have always been cautious of this I have not experienced this until just recently. I also have never seen a publication that describes these effects. In my setup I have been using a membrane-targeted form of citrine I made by adding the Ras CAAX prenylation site to the C-term of citrine. Unless it is expressed at very low concentrations it causes both obvious morphological defects, and leads to early cell death. I have used a similarly made version of Venus which has a very similar sequence, and not seen these effects, though in a slightly different experiment. Does anyone have more knowledge of what membrane-targeted fluorophores are best. I am considering using a palmitoylation sequence since I have it on hand, but am not sure if that will help. Not sure if it is the fluorophore, the linker or the lipid modification that leads to the problem, and am just generally curious what other people think. |
 
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Ana Gil-Bernabe |
Re: membrane-targeted fluorophores
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Dear Steve, I have used PKH26 (Sigma Aldrich) to label platelets for both in vitro and in vivo (injected in mouse) experiments. It works well, the platelets are still functional and the signal is really bright (565 nm excitation) and lasts long time. They also have the green version, which I have not tried yet. In vivo tracking of platelets: circulating degranulated platelets rapidly lose surface P-selectin but continue to circulate and function. Michelson AD1, Barnard MR, Hechtman HB, MacGregor H, Connolly RJ, Loscalzo J, Valeri CR. Best wishes, Ana (Oxford University, Dpt. Oncology) ________________________________________ From: Confocal Microscopy List [[hidden email]] on behalf of Steve [[hidden email]] Sent: 04 April 2014 19:57 To: [hidden email] Subject: membrane-targeted fluorophores ***** To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** I have used membrane-targeted fluorophores for visualizing neuronal morphology off and on over the years. Some colleagues have warned me about their potential side affects, and although I have always been cautious of this I have not experienced this until just recently. I also have never seen a publication that describes these effects. In my setup I have been using a membrane-targeted form of citrine I made by adding the Ras CAAX prenylation site to the C-term of citrine. Unless it is expressed at very low concentrations it causes both obvious morphological defects, and leads to early cell death. I have used a similarly made version of Venus which has a very similar sequence, and not seen these effects, though in a slightly different experiment. Does anyone have more knowledge of what membrane-targeted fluorophores are best. I am considering using a palmitoylation sequence since I have it on hand, but am not sure if that will help. Not sure if it is the fluorophore, the linker or the lipid modification that leads to the problem, and am just generally curious what other people think. |
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Joachim Goedhart-2 |
Re: membrane-targeted fluorophores
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In reply to this post by sjh
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Dear Steve, There are a few details that are missing to fully understand the issue. You mention that the lipidation motif is from Ras, but which isoform of Ras? I guess that it is the C-terminus of KRas, which is widely used. This motif carries a lot of basic residues and is highly positively charged. It therefore interacts with negatively charged phospholipids at the plasma membrane (PI(4,5)P2, PI(4)P and PA), which is good for plasma membrane localization. However, these lipids are essential modulators of various processes, e.g. interacting directly or indirectly with the cytoskeleton (http://www.ncbi.nlm.nih.gov/pubmed/24534649). Another issue is the probe. GFP variants, certainly YFP, can dimerize when it is concentrated at the surface of the membrane (http://www.ncbi.nlm.nih.gov/pubmed/11988576). So do you know whether you are using monomeric YFP variants (e.g. carrying the A206K mutation)? If these proteins are of the 206A type, dimerization may increase PM interaction (good for localization), thereby competing more strongly with endogenous proteins depend on interaction with the PM via negatively charged lipids. We have some experience with the lipidation motif of Lck which gives very good PM labeling, still it does not seem to interfere with cell morphology. The Lck motif was successfully used in fusion proteins with mTurquoise2 and mVenus (the aa sequence preceding the CDS of the FP we used is MGCVCSSNPELPVAT). However, our expts are mainly performed in HeLa cells, so it might be different in neuronal cells. Best Regards, Joachim Goedhart Section Molecular Cytology SILS - University of Amsterdam The Netherlands |
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lechristophe |
Re: membrane-targeted fluorophores
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In reply to this post by sjh
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Hi Steve, We've been using membrane-associated fluorescent proteins in cultured neurons for several years now, as they nicely delineate neuronal morphology. We use the mainly use EGFP-F (Clontech), which is the 20-aa farnesylation signal of c-Ha-Ras fused to the C-Terminus of EGFP. It does not accumulate in endomembranes when expressing for more than 24 hours, which happens in our system with other "membrane" targeting signals like the neuromodulin aminoterminus. Using nucelofection at the time of plating, we usually get expression for > 10 days with no aggregation and no concentration in endomembranes. Regarding expression levels, when transfecting high-level expression vectors (such as lentiviral expression cassettes with enhancers), we see some morphology changes in highly-expressing neurons, with more filopodias. Regarding fluorescent proteins others than EGFP, we've had a hard time finding FPs for other wavelength channels that behave as nicely as EGFP. Most red FPs tested so far (DsRed2, mRFP, mCherry) tend to aggregate over time, most likely due to their tendency to oligomerize. We recently made an TdTomato-F construct, and it seems to be present in endomembrane more than EGFP after several days of expression. I'd like to test the farnesylated version of FusionRed FP (see http://www.evrogen.com/products/FusionRed/FusionRed_Detailed_description.shtml) which is advertised as equivalent to mCherry, with a lot less aggregation, but I'd be happy to have some feedback form people using it before paying for the plasmid. In the blue channel, we also tested an mTagBFP2-F (blue FP), which also resulted in lots of intracellular labeling. Hope this helps, -- Christophe Leterrier Researcher Axonal Domains Architecture Team CRN2M CNRS UMR 7286 Aix Marseille University, France 2014-04-04 20:57 GMT+02:00 Steve <[hidden email]>: > ***** > To join, leave or search the confocal microscopy listserv, go to: > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy > Post images on http://www.imgur.com and include the link in your posting. > ***** > > I have used membrane-targeted fluorophores for visualizing neuronal > morphology > off and on over the years. Some colleagues have warned me about their > potential > side affects, and although I have always been cautious of this I have not > experienced this until just recently. I also have never seen a publication > that > describes these effects. > > In my setup I have been using a membrane-targeted form of citrine I made by > adding the Ras CAAX prenylation site to the C-term of citrine. Unless it is > expressed at very low concentrations it causes both obvious morphological > defects, and leads to early cell death. I have used a similarly made > version of > Venus which has a very similar sequence, and not seen these effects, > though in a > slightly different experiment. > > Does anyone have more knowledge of what membrane-targeted fluorophores are > best. I am considering using a palmitoylation sequence since I have it on > hand, > but am not sure if that will help. Not sure if it is the fluorophore, the > linker or the > lipid modification that leads to the problem, and am just generally > curious what > other people think. > |
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lechristophe |
Re: membrane-targeted fluorophores
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** I should add that the nucleofection/long term expression in hippocampal neurons in a quite stringent test for the quality of an FP, as it is very sensitive to toxicity, aggregation and mislocalization tendencies. Also, it is simpler and faster than in-vivo tests using viruses. If you have a red or blue, soluble or membrane-targeted FP that you think is good, I'd be happy to try it, and share the results with you or the broader audience of the list. Thanks, -- Christophe Leterrier Researcher Axonal Domains Architecture Team CRN2M CNRS UMR 7286 Aix Marseille University, France 2014-04-07 9:33 GMT+02:00 Christophe Leterrier < [hidden email]>: > Hi Steve, > > We've been using membrane-associated fluorescent proteins in cultured > neurons for several years now, as they nicely delineate neuronal > morphology. We use the mainly use EGFP-F (Clontech), which is the 20-aa > farnesylation signal of c-Ha-Ras fused to the C-Terminus of EGFP. It does > not accumulate in endomembranes when expressing for more than 24 hours, > which happens in our system with other "membrane" targeting signals like > the neuromodulin aminoterminus. Using nucelofection at the time of plating, > we usually get expression for > 10 days with no aggregation and no > concentration in endomembranes. > > Regarding expression levels, when transfecting high-level expression > vectors (such as lentiviral expression cassettes with enhancers), we see > some morphology changes in highly-expressing neurons, with more filopodias. > Regarding fluorescent proteins others than EGFP, we've had a hard time > finding FPs for other wavelength channels that behave as nicely as EGFP. > Most red FPs tested so far (DsRed2, mRFP, mCherry) tend to aggregate over > time, most likely due to their tendency to oligomerize. We recently made an > TdTomato-F construct, and it seems to be present in endomembrane more than > EGFP after several days of expression. I'd like to test the farnesylated > version of FusionRed FP (see > http://www.evrogen.com/products/FusionRed/FusionRed_Detailed_description.shtml) > which is advertised as equivalent to mCherry, with a lot less aggregation, > but I'd be happy to have some feedback form people using it before paying > for the plasmid. In the blue channel, we also tested an mTagBFP2-F (blue > FP), which also resulted in lots of intracellular labeling. > > Hope this helps, > > -- > Christophe Leterrier > Researcher > Axonal Domains Architecture Team > CRN2M CNRS UMR 7286 > Aix Marseille University, France > > > > 2014-04-04 20:57 GMT+02:00 Steve <[hidden email]>: > > ***** >> To join, leave or search the confocal microscopy listserv, go to: >> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy >> Post images on http://www.imgur.com and include the link in your posting. >> ***** >> >> I have used membrane-targeted fluorophores for visualizing neuronal >> morphology >> off and on over the years. Some colleagues have warned me about their >> potential >> side affects, and although I have always been cautious of this I have not >> experienced this until just recently. I also have never seen a >> publication that >> describes these effects. >> >> In my setup I have been using a membrane-targeted form of citrine I made >> by >> adding the Ras CAAX prenylation site to the C-term of citrine. Unless it >> is >> expressed at very low concentrations it causes both obvious morphological >> defects, and leads to early cell death. I have used a similarly made >> version of >> Venus which has a very similar sequence, and not seen these effects, >> though in a >> slightly different experiment. >> >> Does anyone have more knowledge of what membrane-targeted fluorophores are >> best. I am considering using a palmitoylation sequence since I have it on >> hand, >> but am not sure if that will help. Not sure if it is the fluorophore, the >> linker or the >> lipid modification that leads to the problem, and am just generally >> curious what >> other people think. >> > > |
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In reply to this post by lechristophe
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To join, leave or search the confocal microscopy listserv, go to: http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy Post images on http://www.imgur.com and include the link in your posting. ***** Hi Christophe, Thanks for the information and suggestions. I had assumed that Citrine would behave similarly to EGFP since there isn't that much difference in their sequence, but perhaps that is not true. Unfortunately in my case it would be difficult to see EGFP to label the membrane since I need that color for labeling other structures. I also had a similar issue with membrane targeted red proteins. They were all either too dim or cause side affects. In particular the form of tdtomato we made got stuck in the ER, and disrupted morphology. I had still hoped to try mOrange2 and TagRFP-T, but had heard negative things about both of those have cytotoxic effects. For that reason I decided to switch to doing cyan and yellow proteins since I thought they were generally more amenable to being used as fusion tags. Citrine and mTurquoise2 were the brightest and that is quite important for my work. I am going to try membrane mTurquoise2 since I already have the constructs, hopefully it will work out better than mTagBFP2-F did for you. In regards to expression levels, I am electroporating into the retina constructs expressing fluorescent proteins under the control of a CAG promoter that are only expressed after being processed by Cre. I would expect expression to be quite a bit lower than lentivirus, but have no experience using it so I am not sure. In the retina I start to see obvious deffects in morphology within 48 hours with the Citrine-CAAX, but do not see anything unusual with cytoplasmic tdTomato. I should note that at this point tdTomato is at least 5 times brighter, but since it is a brighter fluorophore it is difficult to compare protein levels. Thank you for the offer to test constructs in hippocampal cultures. First, I am going to try a few different constructs I currently have in my system to see if I can narrow down the issue a little more, but may contact you in the future. thanks, Steve On Mon, Apr 7, 2014 at 3:33 AM, Christophe Leterrier < [hidden email]> wrote: > ***** > To join, leave or search the confocal microscopy listserv, go to: > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy > Post images on http://www.imgur.com and include the link in your posting. > ***** > > Hi Steve, > > We've been using membrane-associated fluorescent proteins in cultured > neurons for several years now, as they nicely delineate neuronal > morphology. We use the mainly use EGFP-F (Clontech), which is the 20-aa > farnesylation signal of c-Ha-Ras fused to the C-Terminus of EGFP. It does > not accumulate in endomembranes when expressing for more than 24 hours, > which happens in our system with other "membrane" targeting signals like > the neuromodulin aminoterminus. Using nucelofection at the time of plating, > we usually get expression for > 10 days with no aggregation and no > concentration in endomembranes. > > Regarding expression levels, when transfecting high-level expression > vectors (such as lentiviral expression cassettes with enhancers), we see > some morphology changes in highly-expressing neurons, with more filopodias. > Regarding fluorescent proteins others than EGFP, we've had a hard time > finding FPs for other wavelength channels that behave as nicely as EGFP. > Most red FPs tested so far (DsRed2, mRFP, mCherry) tend to aggregate over > time, most likely due to their tendency to oligomerize. We recently made an > TdTomato-F construct, and it seems to be present in endomembrane more than > EGFP after several days of expression. I'd like to test the farnesylated > version of FusionRed FP (see > > http://www.evrogen.com/products/FusionRed/FusionRed_Detailed_description.shtml > ) > which is advertised as equivalent to mCherry, with a lot less aggregation, > but I'd be happy to have some feedback form people using it before paying > for the plasmid. In the blue channel, we also tested an mTagBFP2-F (blue > FP), which also resulted in lots of intracellular labeling. > > Hope this helps, > > -- > Christophe Leterrier > Researcher > Axonal Domains Architecture Team > CRN2M CNRS UMR 7286 > Aix Marseille University, France > > > > 2014-04-04 20:57 GMT+02:00 Steve <[hidden email]>: > > > ***** > > To join, leave or search the confocal microscopy listserv, go to: > > http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy > > Post images on http://www.imgur.com and include the link in your > posting. > > ***** > > > > I have used membrane-targeted fluorophores for visualizing neuronal > > morphology > > off and on over the years. Some colleagues have warned me about their > > potential > > side affects, and although I have always been cautious of this I have not > > experienced this until just recently. I also have never seen a > publication > > that > > describes these effects. > > > > In my setup I have been using a membrane-targeted form of citrine I made > by > > adding the Ras CAAX prenylation site to the C-term of citrine. Unless it > is > > expressed at very low concentrations it causes both obvious morphological > > defects, and leads to early cell death. I have used a similarly made > > version of > > Venus which has a very similar sequence, and not seen these effects, > > though in a > > slightly different experiment. > > > > Does anyone have more knowledge of what membrane-targeted fluorophores > are > > best. I am considering using a palmitoylation sequence since I have it on > > hand, > > but am not sure if that will help. Not sure if it is the fluorophore, the > > linker or the > > lipid modification that leads to the problem, and am just generally > > curious what > > other people think. > > > |
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