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Subject:	Re: Multiphoton - femto vs pico
From:	Patrick Van Oostveldt <[log in to unmask]>
Reply To:	Confocal Microscopy List <[log in to unmask]>
Date:	Wed, 14 Oct 2009 20:18:22 +0200
Content-Type:	text/plain
Parts/Attachments:	text/plain (141 lines)

Dear Friends,

I like to express my sympathy witk Alberto.
Indeed as he stated a lot of patenting has retarded TPE. The pitty  
thing is that our universities purge us to do research and validate  
our research with patents, and the results is that to continu research  
we need spend money to pay the royalties of our collegas at the  
university.

In this way, the snake is byting its tail.

Greetings hut not seeing a reasonable solution

Patrick

Quoting Alberto Diaspro <[log in to unmask]>:

> Friends
> I think that everything is really simpler. Removing the crystal is a
> simple operation and re-alignement as well.
> I agree that fs is not always better than ps, this can depend on your
> own need.
>
> We performed imaging both using ps and fs. I do not have any strange
> patent issue, I simply try to make research. I fully understand all the
> patent issues and I do respect them, even if I continue thinking that
> the TPE patent blocked research in the field for some years with
> exceptions. It is well now that ALL microscopy companies can provide
> systems that can be adapted for multiphoton imaging including SHG
> etc... It is also very well known that in some cases there is the need
> for special techniques but people managing the microscopy lab do not
> have resources or time that can be devoted to users, bright users, that
> do not want to be active part of the image formation process having
> their own research plan. I think that any attempt of perfoming
> microscopy imaging has to be helped and favoured, when possible.
>
> This list is a great source of help, so please, make your experimental
> designs without thinking about patents, ask your questions...get the
> answers...not always you can get the right one but everything can help
> growth ...
> All the best
> Alby
>
>
> On Oct 13, 2009, at 5:26 PM, Craig Brideau wrote:
>
>> You must have some strange patent issues.  I am not a lawyer, so take
>> what I say with a grain of salt, however it seems that as long as it
>> is for use in your own lab and you are not selling a product involving
>> fs lasers or otherwise profiting then you should be within your rights
>> to simply remove the stretcher block from your system.
>>
>> Craig
>>
>>
>> On Tue, Oct 13, 2009 at 7:26 AM, Evangelos   
>> <[log in to unmask]> wrote:
>>>    Femto is not always necessarily better.   You can safely use more
>>> average power with picosecond compared to femtosecond to go deep into brain
>>> or muscle tissue.  I have found that picosecond is /sometimes/ better than
>>> femtosecond, even for SHG.  Femtosecond will give more initial signal but
>>> picosecond signal will stay constant, longer, at the same power, in tissue.
>>> Also, for our confocal core's speciality: CARS microscopy, picosecond is
>>> far superior in that it matches the vibrational linewidths and doesn't dump
>>> a lot of energy in a broad spectral region like femtosecond pulses.
>>> Dispersion is far less of a problem with pico and not as much need to
>>> pre-comp, but I do believe for THG, and if you have very weak 2-photon
>>> signal you would have to used pre-chirped compressed femtosecond pulses,
>>> with SHG on collagen, 2-photon with more average power, and CARS you're ok
>>> with pico, otherwise you need femto.
>>>
>>> Best,
>>> Evangelos
>>>
>>> Advanced Biological Imaging Scientist
>>> Harvard Center for Nanoscale Systems
>>> 11 Oxford Street
>>> Cambridge, MA 02138
>>>
>>> Manja Schubert wrote:
>>>>
>>>> Dear Confocal list members,
>>>>
>>>> I have a question to multiphoton technology - femto second IR laser versus
>>>> pico second IR laser.
>>>> We run in following problem. We have a femto second laser but because of
>>>> patent law we can use it only with attenuation filter and a pulse  
>>>>  stretcher
>>>> meaning in the end we scanning with a pico second IR laser.
>>>>
>>>> Has anyone experienced how that effect the scanning outcome? For example,
>>>> the possible deepness of the scan. Any thoughts are highly appreciated.
>>>>
>>>> Many thanks in advance!
>>>>
>>>> Cheers,
>>>> Manja
>>>>
>>>> Dr. Manja Schubert
>>>> University of Bergen
>>>> Department of Biomedicine
>>>> Jonas Lies  vei 91
>>>> 5009 Bergen
>>>> Norway
>>>> Tel:+47-55 58 67 15
>>>
>
> ----------------------------------------
> Alberto Diaspro
> Head, Nanophysics Unit
> Senior Scientist
> The Italian Institute of Technology -IIT
> Via Morego, 30
> 16163 - Genova (Italy)
> phone: +39 010 71781503
> mobile: +393666719968
> fax:   +39 010 720321
> http://www.iit.it
> [log in to unmask]
>
> Professor of Applied Physics
> Department of Physics
> University of Genova
> Via Dodecaneso, 33
> 16146 Genova - Italy
> tel.  +39 010 353 6426
> fax. +39 010 314218
> http://www.lambs.it
> [log in to unmask]
> -------------------------------------------------------



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