advice wanted

> On 20 May 2015, at 15:30, Maria Y. Boulina <[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.
> *****
>
> Folks,
>
> I need your advice on what to do with a manuscript. The story is, we have been working
> on a quantification protocol for a while with a student on her large-scale imaging project.
> We spent some brain power on it, so at the end, we have decided to publish it as a small
> methods paper. the novelty of our approach was applying the Nyquist sampling rate to
> the target object size, rather than the confocal system output AND adequate post-
> processing. we have shown that 1)our suggested algorithm works well in terms of
> preserving the number of counts acquired, compared to higher sampling rates; and allows
> to  keep image size/sampling density/imaging time about several fold lower than you
> would do standard 2)if you neglect proper sampling rates (linked to the object size!) or
> skip processing, your results suck.
>
> we have sent the paper to two journals, and received three sets of comments
>
> reviewer 1: overall correct, but...nothing new .. AND(!!)... In many studies,
> photobleaching is a major determinant of the spatial sampling rate to use
>
> other journal
>
> reviewer 2:
> ..a pipeline for speckle counting on the CellProfiler example page that seems relevant...
> and..the use of passive voice throughout makes it a difficult and dry read..
>
> reviewer 3:
>
> The authors fail to demonstrate that using this method increases the accuracy of their
> quantitation (We were aiming at preserving the accuracy and minimizing the effort!!).
>
> This method is not broadly applicable (???, almost  every lab has to quantify images).  
>
> My main idea behind submitting the manuscript was, that its always nice to have an
> example of a working protocol, and sampling rate is something often neglected (see
> comments from reviewer 1). I have seen tons of very smart grad students, who need to
> do quantification, but end up performing manual counting on their images, since adapting
> existing protocols is beyond their available effort. On the other hand, I am personally not
> qualified to go deep into physics and math behind sampling according to the PSF of the
> system vs sampling based on object density. However, I know that sampling below
> Nyquist is hot in medical imaging field now.
>
> I can not publish the full method within the main paper from the study. Quit? Try other
> microscopy journals? Publish on the Core's webpage?

> *****
> 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.
> *****
>
> Folks,
>
> I need your advice on what to do with a manuscript. The story is, we have
> been working
> on a quantification protocol for a while with a student on her large-scale
> imaging project.
> We spent some brain power on it, so at the end, we have decided to publish
> it as a small
> methods paper. the novelty of our approach was applying the Nyquist
> sampling rate to
> the target object size, rather than the confocal system output AND
> adequate post-
> processing. we have shown that 1)our suggested algorithm works well in
> terms of
> preserving the number of counts acquired, compared to higher sampling
> rates; and allows
> to  keep image size/sampling density/imaging time about several fold lower
> than you
> would do standard 2)if you neglect proper sampling rates (linked to the
> object size!) or
> skip processing, your results suck.
>
> we have sent the paper to two journals, and received three sets of comments
>
> reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
> studies,
> photobleaching is a major determinant of the spatial sampling rate to use
>
> other journal
>
> reviewer 2:
> ..a pipeline for speckle counting on the CellProfiler example page that
> seems relevant...
> and..the use of passive voice throughout makes it a difficult and dry
> read..
>
> reviewer 3:
>
> The authors fail to demonstrate that using this method increases the
> accuracy of their
> quantitation (We were aiming at preserving the accuracy and minimizing the
> effort!!).
>
> This method is not broadly applicable (???, almost  every lab has to
> quantify images).
>
> My main idea behind submitting the manuscript was, that its always nice to
> have an
> example of a working protocol, and sampling rate is something often
> neglected (see
> comments from reviewer 1). I have seen tons of very smart grad students,
> who need to
> do quantification, but end up performing manual counting on their images,
> since adapting
> existing protocols is beyond their available effort. On the other hand, I
> am personally not
> qualified to go deep into physics and math behind sampling according to
> the PSF of the
> system vs sampling based on object density. However, I know that sampling
> below
> Nyquist is hot in medical imaging field now.
>
> I can not publish the full method within the main paper from the study.
> Quit? Try other
> microscopy journals? Publish on the Core's webpage?
>

> *****
> 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.
> *****
>
> Have you considered an Engineering journal like SPIE Biophotonics? They
> might be more appreciative of a sampling technique, and since they went
> open access their impact factor has started to climb a bit. It was fairly
> exclusive before going open.
>
> Craig
> On May 20, 2015 8:32 AM, "Maria Y. Boulina" <[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.
>> *****
>>
>> Folks,
>>
>> I need your advice on what to do with a manuscript. The story is, we have
>> been working
>> on a quantification protocol for a while with a student on her large-scale
>> imaging project.
>> We spent some brain power on it, so at the end, we have decided to publish
>> it as a small
>> methods paper. the novelty of our approach was applying the Nyquist
>> sampling rate to
>> the target object size, rather than the confocal system output AND
>> adequate post-
>> processing. we have shown that 1)our suggested algorithm works well in
>> terms of
>> preserving the number of counts acquired, compared to higher sampling
>> rates; and allows
>> to  keep image size/sampling density/imaging time about several fold lower
>> than you
>> would do standard 2)if you neglect proper sampling rates (linked to the
>> object size!) or
>> skip processing, your results suck.
>>
>> we have sent the paper to two journals, and received three sets of comments
>>
>> reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
>> studies,
>> photobleaching is a major determinant of the spatial sampling rate to use
>>
>> other journal
>>
>> reviewer 2:
>> ..a pipeline for speckle counting on the CellProfiler example page that
>> seems relevant...
>> and..the use of passive voice throughout makes it a difficult and dry
>> read..
>>
>> reviewer 3:
>>
>> The authors fail to demonstrate that using this method increases the
>> accuracy of their
>> quantitation (We were aiming at preserving the accuracy and minimizing the
>> effort!!).
>>
>> This method is not broadly applicable (???, almost  every lab has to
>> quantify images).
>>
>> My main idea behind submitting the manuscript was, that its always nice to
>> have an
>> example of a working protocol, and sampling rate is something often
>> neglected (see
>> comments from reviewer 1). I have seen tons of very smart grad students,
>> who need to
>> do quantification, but end up performing manual counting on their images,
>> since adapting
>> existing protocols is beyond their available effort. On the other hand, I
>> am personally not
>> qualified to go deep into physics and math behind sampling according to
>> the PSF of the
>> system vs sampling based on object density. However, I know that sampling
>> below
>> Nyquist is hot in medical imaging field now.
>>
>> I can not publish the full method within the main paper from the study.
>> Quit? Try other
>> microscopy journals? Publish on the Core's webpage?
>>
>

> *****
> 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 would also look at PLoS One - they are not supposed to evaluate on
> impact, just on scientific correctness.  The one paper I published there
> was a fairly easy process. It is open access with publishing charges.
>
> Kurt
>
>
> On 5/20/2015 8:22 AM, Craig Brideau 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.
>> *****
>>
>> Have you considered an Engineering journal like SPIE Biophotonics? They
>> might be more appreciative of a sampling technique, and since they went
>> open access their impact factor has started to climb a bit. It was fairly
>> exclusive before going open.
>>
>> Craig
>> On May 20, 2015 8:32 AM, "Maria Y. Boulina" <[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.
>>> *****
>>>
>>> Folks,
>>>
>>> I need your advice on what to do with a manuscript. The story is, we have
>>> been working
>>> on a quantification protocol for a while with a student on her
>>> large-scale
>>> imaging project.
>>> We spent some brain power on it, so at the end, we have decided to
>>> publish
>>> it as a small
>>> methods paper. the novelty of our approach was applying the Nyquist
>>> sampling rate to
>>> the target object size, rather than the confocal system output AND
>>> adequate post-
>>> processing. we have shown that 1)our suggested algorithm works well in
>>> terms of
>>> preserving the number of counts acquired, compared to higher sampling
>>> rates; and allows
>>> to  keep image size/sampling density/imaging time about several fold
>>> lower
>>> than you
>>> would do standard 2)if you neglect proper sampling rates (linked to the
>>> object size!) or
>>> skip processing, your results suck.
>>>
>>> we have sent the paper to two journals, and received three sets of
>>> comments
>>>
>>> reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
>>> studies,
>>> photobleaching is a major determinant of the spatial sampling rate to use
>>>
>>> other journal
>>>
>>> reviewer 2:
>>> ..a pipeline for speckle counting on the CellProfiler example page that
>>> seems relevant...
>>> and..the use of passive voice throughout makes it a difficult and dry
>>> read..
>>>
>>> reviewer 3:
>>>
>>> The authors fail to demonstrate that using this method increases the
>>> accuracy of their
>>> quantitation (We were aiming at preserving the accuracy and minimizing
>>> the
>>> effort!!).
>>>
>>> This method is not broadly applicable (???, almost  every lab has to
>>> quantify images).
>>>
>>> My main idea behind submitting the manuscript was, that its always nice
>>> to
>>> have an
>>> example of a working protocol, and sampling rate is something often
>>> neglected (see
>>> comments from reviewer 1). I have seen tons of very smart grad students,
>>> who need to
>>> do quantification, but end up performing manual counting on their images,
>>> since adapting
>>> existing protocols is beyond their available effort. On the other hand, I
>>> am personally not
>>> qualified to go deep into physics and math behind sampling according to
>>> the PSF of the
>>> system vs sampling based on object density. However, I know that sampling
>>> below
>>> Nyquist is hot in medical imaging field now.
>>>
>>> I can not publish the full method within the main paper from the study.
>>> Quit? Try other
>>> microscopy journals? Publish on the Core's webpage?
>>>
>>>
>>
>
> --
> Kurt Thorn
> Associate Professor
> Director, Nikon Imaging Center
> http://thornlab.ucsf.edu/
> http://nic.ucsf.edu/blog/
>

> *****
> 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 would also look at PLoS One - they are not supposed to evaluate on
> impact, just on scientific correctness.  The one paper I published there
> was a fairly easy process. It is open access with publishing charges.
>
> Kurt
>
>
> On 5/20/2015 8:22 AM, Craig Brideau 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.
>> *****
>>
>> Have you considered an Engineering journal like SPIE Biophotonics? They
>> might be more appreciative of a sampling technique, and since they went
>> open access their impact factor has started to climb a bit. It was fairly
>> exclusive before going open.
>>
>> Craig
>> On May 20, 2015 8:32 AM, "Maria Y. Boulina" <[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.
>>> *****
>>>
>>> Folks,
>>>
>>> I need your advice on what to do with a manuscript. The story is, we have
>>> been working
>>> on a quantification protocol for a while with a student on her
>>> large-scale
>>> imaging project.
>>> We spent some brain power on it, so at the end, we have decided to
>>> publish
>>> it as a small
>>> methods paper. the novelty of our approach was applying the Nyquist
>>> sampling rate to
>>> the target object size, rather than the confocal system output AND
>>> adequate post-
>>> processing. we have shown that 1)our suggested algorithm works well in
>>> terms of
>>> preserving the number of counts acquired, compared to higher sampling
>>> rates; and allows
>>> to  keep image size/sampling density/imaging time about several fold
>>> lower
>>> than you
>>> would do standard 2)if you neglect proper sampling rates (linked to the
>>> object size!) or
>>> skip processing, your results suck.
>>>
>>> we have sent the paper to two journals, and received three sets of
>>> comments
>>>
>>> reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
>>> studies,
>>> photobleaching is a major determinant of the spatial sampling rate to use
>>>
>>> other journal
>>>
>>> reviewer 2:
>>> ..a pipeline for speckle counting on the CellProfiler example page that
>>> seems relevant...
>>> and..the use of passive voice throughout makes it a difficult and dry
>>> read..
>>>
>>> reviewer 3:
>>>
>>> The authors fail to demonstrate that using this method increases the
>>> accuracy of their
>>> quantitation (We were aiming at preserving the accuracy and minimizing
>>> the
>>> effort!!).
>>>
>>> This method is not broadly applicable (???, almost  every lab has to
>>> quantify images).
>>>
>>> My main idea behind submitting the manuscript was, that its always nice
>>> to
>>> have an
>>> example of a working protocol, and sampling rate is something often
>>> neglected (see
>>> comments from reviewer 1). I have seen tons of very smart grad students,
>>> who need to
>>> do quantification, but end up performing manual counting on their images,
>>> since adapting
>>> existing protocols is beyond their available effort. On the other hand, I
>>> am personally not
>>> qualified to go deep into physics and math behind sampling according to
>>> the PSF of the
>>> system vs sampling based on object density. However, I know that sampling
>>> below
>>> Nyquist is hot in medical imaging field now.
>>>
>>> I can not publish the full method within the main paper from the study.
>>> Quit? Try other
>>> microscopy journals? Publish on the Core's webpage?
>>>
>>>
>>
>
> --
> Kurt Thorn
> Associate Professor
> Director, Nikon Imaging Center
> http://thornlab.ucsf.edu/
> http://nic.ucsf.edu/blog/
>

> *****
> 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 Maria
>
> Its is true that there is little room for methodologies developed in core
> facilities. They might be of great value for the community but
> scientifically not so relevant or new.
>
> This was one of the reasons why we just release an award targeting exactly
> this kind of work. The award has international and independent reviewers.
> Therefore, on top of the prize (a macbook for you and our software for 2
> years for your institution), there is also the international recognition.
>
> More details at
> cirklo.org  (follow the prize link)
>
> Good luck with your application!
>
> All the best
> Nuno Moreno
>
> > On 20 May 2015, at 15:30, Maria Y. Boulina <[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.
> > *****
> >
> > Folks,
> >
> > I need your advice on what to do with a manuscript. The story is, we
> have been working
> > on a quantification protocol for a while with a student on her
> large-scale imaging project.
> > We spent some brain power on it, so at the end, we have decided to
> publish it as a small
> > methods paper. the novelty of our approach was applying the Nyquist
> sampling rate to
> > the target object size, rather than the confocal system output AND
> adequate post-
> > processing. we have shown that 1)our suggested algorithm works well in
> terms of
> > preserving the number of counts acquired, compared to higher sampling
> rates; and allows
> > to  keep image size/sampling density/imaging time about several fold
> lower than you
> > would do standard 2)if you neglect proper sampling rates (linked to the
> object size!) or
> > skip processing, your results suck.
> >
> > we have sent the paper to two journals, and received three sets of
> comments
> >
> > reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
> studies,
> > photobleaching is a major determinant of the spatial sampling rate to use
> >
> > other journal
> >
> > reviewer 2:
> > ..a pipeline for speckle counting on the CellProfiler example page that
> seems relevant...
> > and..the use of passive voice throughout makes it a difficult and dry
> read..
> >
> > reviewer 3:
> >
> > The authors fail to demonstrate that using this method increases the
> accuracy of their
> > quantitation (We were aiming at preserving the accuracy and minimizing
> the effort!!).
> >
> > This method is not broadly applicable (???, almost  every lab has to
> quantify images).
> >
> > My main idea behind submitting the manuscript was, that its always nice
> to have an
> > example of a working protocol, and sampling rate is something often
> neglected (see
> > comments from reviewer 1). I have seen tons of very smart grad students,
> who need to
> > do quantification, but end up performing manual counting on their
> images, since adapting
> > existing protocols is beyond their available effort. On the other hand,
> I am personally not
> > qualified to go deep into physics and math behind sampling according to
> the PSF of the
> > system vs sampling based on object density. However, I know that
> sampling below
> > Nyquist is hot in medical imaging field now.
> >
> > I can not publish the full method within the main paper from the study.
> Quit? Try other
> > microscopy journals? Publish on the Core's webpage?
>

> *****
> 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.
> *****
>
> Have you considered an Engineering journal like SPIE Biophotonics? They
> might be more appreciative of a sampling technique, and since they went
> open access their impact factor has started to climb a bit. It was fairly
> exclusive before going open.
>
> Craig
> On May 20, 2015 8:32 AM, "Maria Y. Boulina" <[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.
> > *****
> >
> > Folks,
> >
> > I need your advice on what to do with a manuscript. The story is, we have
> > been working
> > on a quantification protocol for a while with a student on her
> large-scale
> > imaging project.
> > We spent some brain power on it, so at the end, we have decided to
> publish
> > it as a small
> > methods paper. the novelty of our approach was applying the Nyquist
> > sampling rate to
> > the target object size, rather than the confocal system output AND
> > adequate post-
> > processing. we have shown that 1)our suggested algorithm works well in
> > terms of
> > preserving the number of counts acquired, compared to higher sampling
> > rates; and allows
> > to  keep image size/sampling density/imaging time about several fold
> lower
> > than you
> > would do standard 2)if you neglect proper sampling rates (linked to the
> > object size!) or
> > skip processing, your results suck.
> >
> > we have sent the paper to two journals, and received three sets of
> comments
> >
> > reviewer 1: overall correct, but...nothing new .. AND(!!)... In many
> > studies,
> > photobleaching is a major determinant of the spatial sampling rate to use
> >
> > other journal
> >
> > reviewer 2:
> > ..a pipeline for speckle counting on the CellProfiler example page that
> > seems relevant...
> > and..the use of passive voice throughout makes it a difficult and dry
> > read..
> >
> > reviewer 3:
> >
> > The authors fail to demonstrate that using this method increases the
> > accuracy of their
> > quantitation (We were aiming at preserving the accuracy and minimizing
> the
> > effort!!).
> >
> > This method is not broadly applicable (???, almost  every lab has to
> > quantify images).
> >
> > My main idea behind submitting the manuscript was, that its always nice
> to
> > have an
> > example of a working protocol, and sampling rate is something often
> > neglected (see
> > comments from reviewer 1). I have seen tons of very smart grad students,
> > who need to
> > do quantification, but end up performing manual counting on their images,
> > since adapting
> > existing protocols is beyond their available effort. On the other hand, I
> > am personally not
> > qualified to go deep into physics and math behind sampling according to
> > the PSF of the
> > system vs sampling based on object density. However, I know that sampling
> > below
> > Nyquist is hot in medical imaging field now.
> >
> > I can not publish the full method within the main paper from the study.
> > Quit? Try other
> > microscopy journals? Publish on the Core's webpage?
> >
>