and detailed contacts, please visit
www.biocenter.helsinki.fi/bi/recruit or contact bi‐direc...@helsinki.fi.
www.biocenter.helsinki.fi/bi
Tommi Kajander, Ph.D.
Team Leader
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1 (P.O. Box 65)
00014
FYI, on behalf of the search committee (see links below):
The Institute of Biotechnology is a leading European research institute within
the University of Helsinki with a mission to increase knowledge in
cross‐disciplinary biology and biotechnology. The Institute has state‐ofthe‐art
facilities
and that the data don't show
> interpretable density in that region.
>
> I would call everything else 'tabloid science'.
>
> Cheers,
> Tim
>
> On 10/24/2014 04:11 PM, Michal Jamroz wrote:
>> Dnia 2014-10-22, o godz. 15:43:18
>> Tommi Kajander
Hi All,
Would anyone know a software to model (just with some kind of random coil) the
amino acid chain for
the assumed flexible disorderd regions between domains, or at one end of
protein? just for illustrative purposes.
Thanks!
Tommi
Dear All,
Can someone sugegst what would be the best options for stereo viewing for macs
currently?
Any good experiences with Stereo-TVs? Other? I would like know the specific
combination (at least
which mac computer etc) if possible to find out something that works.
Thanks,
Tommi
Tommi
A postdoctoral position is available in the Biocenter Finland Crystallization
Core Facility, in the research group of
Dr. Tommi Kajander at the institute of Biotechnology at University of Helsinki,
Finland.
The position is funded for two years starting from September 2014.
The position will
A postdoctoral position in structural biology is available from Sept 2014
earliest in the research group lead by
Tommi Kajander at Institute of Biotechnology, University of Helsinki, Finland.
The position is funded by the Academy of Finland at the Finnish university
salary scale 5.
The
Dear all,
I would be interested in comments/opinions about what is your experience on
which
would be the best mammalian cell culture vector/cell line/medium combination
for transient
expression to get the best yields. Depends, of course, but anyway obviously
there are
differences, HEKs are sup
Ok. you filled my mailbox the second time today - please do stop sending junk
to the list.
-tommi
On Mar 23, 2013, at 3:59 PM, Wei Feng wrote:
> Dear Steffi,
> Thank you very much for you patient reply!
> I have tried to use your script to convert the map format, but no
> ***omit_map.coeff c
urify with gel filtration column. However,
>> the one I am currently working on seems to be very picky. If you
>> have any suggestion regarding to my problems, I will be thankful.
>>
>> Best regards,
>>
>
> - --
> - --
> Dr Tim Gruene
> Institu
us overexpression, you can try:
> SOLpro in http://scratch.proteomics.ics.uci.edu/
> Or
> http://mips.helmholtz-muenchen.de/proso/proso.seam
> http://www.biotech.ou.edu/
>
> Thanks,
> Debanu
>
>
> -Original Message-
> From: CCP4 bulletin board [mailto:CCP4B
Hi all,
Does anyone a program/paper that would give some quantitative estimate for
protein solubility based on surface property analysis?
(excluding obvious things such as integral membrane / TM regions)
Best
Tommi
well, actually i recommend having a look at the old but good scalepack manual
for why Rmerge is inferior..
(i thought this was clear long ago.. so i am bit amazed that this discussio is
still alive and kicking..)
question of where to cut, is a different one and thats where the recent papers
an
if you have "peek" surface or titanium parts (if i recall right) there are no
problems with salt solutions.
tommi
On May 30, 2012, at 3:39 AM, aaleshin wrote:
> Back in Iowa State University we used Waters HPLC for protein purification
> during many years without noticeable damage to the sta
, but i havent done a systemic test.
(which now seems like a good idea.. as the samples are _quite
precious_ and i certainly want to keep a track of them all the way through)
--Observations?
(and yes we do 2 ul samples with nanodrop.)
Thanks in advance,
Best,
T.
Tommi Kajander, Ph.D
if you use oil do direct dry Paratone-N, with paraffin oil is not as good.
Li-salts should
work also - i would almos imgaine you can freeze directly from so high
(NH4)2SO4 conc.
but perhaps not. little bit (10%) glycerol probably does it also..
Tommi
On Feb 6, 2012, at 12:55 AM, Vineet Gaur wr
looks like.)
--would like to be able to correct this.
Thanks for comments.
Cheers,
Tommi
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
would need to get the averaging
to work first... )
Tommi Kajander, Ph.D., Docent
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
On Dec 21, 2011, at 12:56 PM
...)
favorite programs for NCS averiging?? DM obviously, and solomon doesnt do it.
Others that do it
(with out a PDB or atoms to derive it from, but rather operators)
Thanks,
Tommi
Tommi Kajander, Ph.D., Docent
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
rsc.org/shop/books/2008/9780854042722.asp
>>>
>>
>>
>>
>> Mark J van Raaij
>> Laboratorio M-4
>> Dpto de Estructura de Macromoléculas
>> Centro Nacional de Biotecnología - CSIC
>> c/Darwin 3, Campus Cantoblanco
>> 28049 Madrid
>> tel. 91 585 4616
>
this mid-point
> plus other pairs (symmetry-equivalent) ... ?
>
> Cheers
>
> Clemens
>
> On Fri, Nov 25, 2011 at 10:55:49AM +0200, Tommi Kajander wrote:
>> Hi, anybody have a script to to find a translation for 2-fold NCS (rotaion)
>> axis based on the center of NCS
Hi, anybody have a script to to find a translation for 2-fold NCS (rotaion)
axis based on the center of NCS symmetry..?? (ie to the midpoint of line
between to heavy atoms)
This search option doenst seem to be endoed anywhere (why??) ...stupid me...
Thanks,
tommi
Hi, if you change crystal infro (SG P2 --> P21) and column labels at the same
time F col label (like FP) cant be changed to anything else
at the same time for whatever reason... at least i had this prob. ccp4 vs 6.2
tommi
ificant band broadening when using these small
columns with a regular fplc (rather than Akta's microFPLC)?
I would greatly appreciate your comments! Many thanks...
Bests,
Alex
.
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
.
Can you do the toothbrush test with SYBR Safe?
JPK
***
Jacob Pearson Keller
Northwestern University
Medical Scientist Training Program
cel: 773.608.9185
email: j-kell...@northwestern.edu
***
Tommi Kajander, P
f Biochemistry
Ludwig-Maximilians-Universität München
Feodor-Lynen-Str. 25
D-81377 Munich
Germany
Phone: +49-89-2180-76845
Fax:+49-89-2180-76999
E-mail: kostr...@genzentrum.lmu.de
WWW:www.genzentrum.lmu.de
***
Tommi Kajander,
HI, looks like - at least for us on Mac OSX (both snow leopard and
Lion), in the latest CCP4 (and already previous versions of CCP4)
xplot84 is broken,
the .plt plots dont work (ie programs that produce these are useless
for that purpose...). ...worth fixing perhaps?
Tommi
Tommi Kajander
I would add that there are some issues with air, you have to be careful with
nanodrop that the path is ok, and also if concentrations are low, <1 mg/ml for
instance, i am not sure one can trust it - compare 50 ul 1 cm path results with
nano at 0.5-1 mg/ml... i get inconsistency there.. its good
at 04:36:59PM +0300, tommi kajander wrote:
Dear all,
Does anyone have suggestions for 6 Å resolution phasing with large
number (40-50) Se sites (SAD so far)??
Thanks a bunch,
Tommi
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Bioph
Dear all,
Does anyone have suggestions for 6 Å resolution phasing with large
number (40-50) Se sites (SAD so far)??
Thanks a bunch,
Tommi
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O
.
I will prompty post a summary of the thread.
Best regards
Savvas et al.
Savvas Savvides
Unit for Structural Biology @ L-ProBE
Ghent University
K.L. Ledeganckstraat 35, 9000 Ghent, Belgium
Tel/SMS/texting +32 (0)472 928 519
Skype: savvas.savvides_skype
http://www.LProBE.ugent.be/x
gram
cel: 773.608.9185
email: j-kell...@northwestern.edu<mailto:j-kell...@northwestern.edu>
***
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
9185
email: j-kell...@northwestern.edu
***
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
Netherlands
Tel. +31-30-253-2383
--
Xiaoguang Xue, PhD student
Utrecht University
Crystal & Structural Chemistry
Padualaan 8. Room N807
3584 CH Utrecht
The Netherlands
Tel. +31-30-253-2383
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikin
would be happy to hear if anyone had similar problems
Thanks!
tommi
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-
of Biochemistry
Albert Einstein College of Medicine
1300 Morris Park Ave
Bronx, NY 10461
phone 718-430-2745
yu...@medusa.vioc.aecom.yu.edu
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
,
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 Helsinki, Finland
Tel. +358-9-191 58903
Fax +358-9-191 59940
I think the likely reason here are the points where you did the
mutations having adverse effects
- how do the mutants behave without labeling? this would be of course
an important control...
-Tommi
On 25.1.2011, at 12.52, Paula Salgado wrote:
Dear Abhilash
You could try an alternative la
902-149
e-mail: fabio.dallanto...@embl-hamburg.de
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
stupid,
any help will be appreciated!!
Best wishes,
Xiaopeng Hu
Harry
--
Dr Harry Powell,
MRC Laboratory of Molecular Biology,
Hills Road,
Cambridge,
CB2 0QH
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
300mM
NaCl
3.Before making complex I spun the protein @14,000rpm 10min.
the complex solution is clear.
Regards
Dilip
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9
Hello all,
Would anyone happen to have a met auxotroph S. cerevisaea strain at
hand that you
could send some of to us for testing Semet labelling?
Thanks very much!
Regards,
Tommi
Tommi Kajander, Ph.D.,
Macromolecular X-ray Crystallography
Research Program in Structural Biology and
mbus, OH 43210-1185
(614) 859-5743 phone (Google Voice)
(614) 292-1685 fax
magli...@chemistry.ohio-state.edu
http://www.chemistry.ohio-state.edu/~magliery
Tommi Kajander, Ph.D., Docent
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O.
--
When the Way is forgotten duty and justice appear;
Then knowledge and wisdom are born along with hypocrisy.
When harmonious relationships dissolve then respect and devotion arise;
When a nation falls to chaos then loyalty and patriotism are born.
------ / Lao Tse /
think overall of the different manufacturers equipments
accuracy, etc...
e.g. viscometer seems rather unnessary to me, as does online DLs..
Thanks for comments,
Tommi
--
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Inst
equipment and filters. So it all pays off only
of you need large scale cultures long-term.
If you are aware of a dry serum-free insect cells medium, please
let me know - I'd love to try it.
Dima
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of He
Padavattan
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
a toolbox of Matlab software.
Thank you in advance,
Azadeh
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street address: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 H
Would the exact analysis of how each of these things were wrong and
fabricated be somewhere
available Would be fair (apart from the known case of C3b) to have
the whole analysis available
instead of just this kind of news feed. I suspect its not obvious by
five minute check in all cases.
very much for comments,
Tommi
Tommi Kajander, Ph.D., Docent
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 Helsinki, Finland
Tel. +358-9-191 58903
t; etc...
(I suggest you take only one zone for the rigid body refinement
because at 6A you only have so many reflections)
Best
Jacques
Le Nov 26, 2009 à 8:32 PM, Tommi Kajander a écrit :
Apologies, i know this is not phenix bb but since i am here (and
not subscr. there), does anyone
know
Apologies, i know this is not phenix bb but since i am here (and not
subscr. there), does anyone
know how to control rigid body ref positions in phenix.refine, i am
trying to do very low res check
(6 Å) with quite many molecules, and they start landing on each other
while the MR solution from
Hi, the latest arpwarp via ccp4 6.1.2 GUI on Mac OS X 10.5 something
does
not work, it wants a sequence file which isnt an option in the GUI...
(you put in the coordinates and update them thats all right?) i just
want to improve
the maps if possible. also the model if possible.. flex-warp didn
Dear all
I was wondering if anyone knows a simple way to generate a missing
loop (strech of amino acids)
really in just some simple manner (no fancy minization necessary, of
course some constraints probably dont
hurt), just for visualization purposes of further simulations etc
thanks!
to
ce does not provide definitive answer, given
that
the interacting residues on the interface are also different.
BTW, we were not able to purify individual domains, so we cannot measure
the
binding affinity by wet lab approaches (so far).
Thank you in advance for your inputs.
--
Best regards,
Joe
ng data."
And I cannot find how to fix this.
It have also one more warning message - * Missing value set to NaN
in input
mtz file
but as I read it is not a problem - mtz is still readable.
I would be glad for any help or advice.
Thanks.
Sergii
P.S. Please, find attached mtz and logs.
Hi,
I have been using a dimer as a search model in MOLREP (there will be
several in AU),
for some reason the program tends to break the dimer into monomers
wihtout asking me..
how is this determined in the program... a more detailed manual would
be nice, also on the output
as the different c
ion a bit easier.
Tim
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 Helsinki, Finland
Tel. +358-9-191 58903
Fax +358-9-191 59940
nks anyway..
tommi
On Sep 13, 2009, at 3:52 PM, Tommi Kajander wrote:
Hi,
off-crystal topic: i was wondering if anyone has a simple solution to
combining e.g. CLUSTAL etc ouput files to format (ie idcodes then 60
residues strech and start again below the same...) ...that has only
one line pe
simply combining lines which start with same set of
characters (ID) but removing the IDs
codes from everyelse but the beginning. i am not much of a script
writer obivously
Thanks a bunch!
Tommi
Tommi Kajander
Structural Biology and Biophysics
Institute of Biotechnology
University of
ble with decent data.
BR
-Original Message-
From: CCP4 bulletin board [mailto:ccp...@jiscmail.ac.uk] On Behalf Of Tommi
Kajander
Sent: Friday, March 20, 2009 3:43 PM
To: CCP4BB@JISCMAIL.AC.UK
Subject: Re: [ccp4bb] Problems with phasing a protein (1300aa)
this cant be true,
in the idea case (
on of 3.3A (Space group I222
or
I212121). But we are having tough time phasing it.
...
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
tommi.kajan...@helsinki.fi
convert the file to either a ccp4 or
cns map file, or a file format that pymol will recognize. I do not
have an .mtz file with the same map coefficients included. Can
anyone help me?
Thanks,
John
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural
For this discussion another relevant reference might be:
The 1.8 A crystal structure of a statically disordered 17 base-pair
RNA duplex: principles of RNA crystal packing and its effect on
nucleic acid structure.
Shah SA, Brunger AT.
J Mol Biol. 1999 Jan 29;285(4):1577-88.
-tommi
On Jan 2
of the opposite case, where the protein is a monomer in
solution (as evident from light scattering, MW determination through
centrifugation, EPR, etc.) but crystallizes as a dimer or higher multimer?
Bernie Santarsiero
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Res
file
with secondary structure assigned from DSSP.
Thanks!
Charu
Mayer lab/NIH
--
MRC National Institute for Medical Research
Division of Molecular Structure
The Ridgeway, NW7 1AA, UK
Email: [EMAIL PROTECTED]
Phone: + 44 208 816 2515
Tommi Kajander, Ph.D.
Structural Biology and Biop
---
>> Chavas Leonard, Ph.D. @ home
>> Research Associate
>> Marie Curie Actions Fellow
>>
>> Faculty of Life Sciences
>> The University of Manchester
>> The Michael Smith Buildi
Also, i think that would be nice if this type of info could be put on
the web, part of the wiki for instance..
if there is some consensus to what works + the typical proteins easily
available.
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of
good enough for demonstration
purposes, so we need more)
Thanks very much!
best,
Tommi
Tommi Kajander, Ph.D.
Structural Biology and Biophysics
Institute of Biotechnology
University of Helsinki
Viikinkaari 1
(P.O. Box 65)
00014 Helsinki
Finland
p. +358-9-19158903
[EMAIL PROTECTED]
ALWAYS OFTEN SOMETIMES RARELY NEVER
Answer:
8) Is there any software you would like to have available in the
computing environment to assist you in molecular model building
and/or
visualization that is not currently available?
Answer:
Thank you for your time.
Tommi Kajander
with regard to what is "guaranteed"--usually you get a mass spec /
HPLC etc
sheets telling you what the real purity is. checking that is certainly
worthwhile.
i would perhaps first try with 95% pure and then if not good enough
purify further.
this purity scale has worked ok for us.
tommi
system
for more efficient recombinant protein production in insect cells.
Protein Expr Purif. 2005 Jul;42(1):211-8
or if i can reach one of the authors is reachable this way and willing
to send some material i would be greatful.
thank you,
tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray
re sample, of course.
>
> Cheers,
>
> --
>
> Roger S. Rowlett
> Professor
> Colgate University Presidential Scholar
> Department of Chemistry
> Colgate University
> 13 Oak Drive
> Hamilton, NY 13346
>
> tel: (315)-228-7245
> ofc: (315)
kindly help me to progress in my experiment.
> Phoebe A. Rice
> Assoc. Prof., Dept. of Biochemistry & Molecular Biology
> The University of Chicago
> phone 773 834 1723
>
http://bmb.bsd.uchicago.edu/Faculty_and_Research/01_Faculty/01_Faculty_Alphabetically.php?faculty_id=123
prove my
> diffraction data?
> This crystal grew in 2.5M Ammonium Sulfate.
>
> Thank you so much.
>
> Ji
>
>
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
P.O. Box 65 (Street
liquid N2, which causes boiling around the crystal immediately after
> plunging.
>
> The best way to freeze things is to put a small container of liquid
> ethane
> or propane into a liquid N2 bowl, and plunge into the ethane/propane
> (this
> methods was suggested ea
---
> >
>
>
> ___
>
> Dr. Christian Biertümpfel
> Laboratory of Molecular Biology
>
> NIDDK/National Institutes of Health phone: +1 301 402 4647
>
ey are secreted into the media.
>
> 1) Baculovirus system
> 2) Drosophila system
>
> Which system would you recommend for high expression and convenience?
> Has anyone ever compared those systems side by side?
>
> Any suggestions or references are greatly appreciated.
>
t; >>
> >> ***
> >> * Clemens Vonrhein, Ph.D. vonrhein AT GlobalPhasing DOT com
> >> *
> >> * Global Phasing Ltd.
> >> * Sheraton House, Castle Park
> >> * Camb
rop size is 3+1 with mother liquor 300
> micro
> lt.Numerous xtals appears and but small is size.Do anyone can share
> their
> experience with Isopropanol as a precipitant and to improve the xtal
> quality
> with other precipitants.All suggestions are welcome.
> Thanx in advance.
glycerol into one of the fractions but that made it even more cloudy
> > (ohh no...).
> >
> > While the protein is dying in the tube, do you have some quick remedy
> > for me? Thanks very much, -J.J.
>
>
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallograp
difference (getting xprep will cost some money so i would like to know
where the difference lies if there is any significant difference??)
Thanks for advice,
Tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of
es
> not bind amylose resin any better with majority flows right through. All
> purification are carried out under standard conditions as mentioned in
> the
> manuals. The protein is soluble and does not precipitate in the columns.
> I
> appreciate and ideas or explanations.
>
&g
size/Mw? is this really
so?
--- of course this may further vary depending on the oligomeric state of the
protein --suppose some neutron scattering studies on model systems might
give the answer --havent looked. just wondering..
-tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallo
europe most relevant)
thanks very much,
tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
PO box 65 (Street address: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 Helsinki, Finland
Tel
Hi,
i would be interested in hints about what would be the best
way to combine & improve SAD phases from two (or several)
non-isomorphous crystals, i can only get reasonable phases from
SHARP so far i think.
(the other set is very poor but has some signal there)
one back as HLs into sharp? or d
Quoting Anastassis Perrakis <[EMAIL PROTECTED]>:
> On Aug 9, 2007, at 15:02, Tommi Kajander wrote:
>
> > so, a) WHAT IS GAMMA??
>
> gamma is possibly the letter of the greek alphabet that has had most
> abuse from scientists.
thats what i thought...
> http:
success to go beyond it by any
meanstweaking parameters in arpwarp now suggestions??)
many thanks...,
tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
PO box 65 (Street address
ed to hear opinions though...)
cheers,
tommi
Quoting Anastassis Perrakis <[EMAIL PROTECTED]>:
>
> On Jul 31, 2007, at 15:24, Tommi Kajander wrote:
>
> > Hi,
> > i would be interested in hearing about people's preferences on
> > programs
> > for doign
cases
where there was some difference to what you started with...
..of course one can always complete and correct by hand but when you are
doing this with phasing iteratively it would be interesting to hear opinions..
thanks,
tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallog
Quoting Priyank Maindola <[EMAIL PROTECTED]>:
> Hello all,
> I am struggling with getting the phases out for my protein. Heavyatom
> database shows that only mercury and samarium have the binding motifs in
> it.
>
> Sodium iodide soak is killing the crystal even as less as 0.2 Molar
> concentra
t; > 20139 Milano
> > Italy
> >
> > tel +39 02 9437 5094
> > fax +39 02 574 303 310
> >
> >
> --------
> >
> >
> >
> > No virus found in this outgoing message.
> &
).
Thanks,
Tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
PO box 65 (Street address: Viikinkaari 1, 4th floor)
University of Helsinki
FIN-00014 Helsinki, Finland
Tel. +358-9-191 58903
Fax +358-9
d 0.5M ammonium sulfate?
> I read from Hampton user guide of heavy atom kit that "high salt
> concentrations are not the ideal medium for heavy atom reactions with
> macromolecules", so is there any type of heavy atom we should avoid
> using? We do not have any experience in
ed NaCl as the salt, in a 4*6 tray, the
> >> [NaCl] is going from 2.0,2.05,2.1,2.15,something like
> >> that and 0.05M does make big difference.I used Urea as the
> >> additive in this case ( 25 m ~ 100 mM) and tried
> >> 2+2,3+1,3+2, 3+1 ( 3 uL prot
where the
> > protein density and ligand density can be distinguished at such high
> > B-factors. Does anyone have any suggestions if there is something
> going
> > wrong here?
> >
> > Thanks,
> >
> > George
> >
> >
> >
>
_
Hi, would anyone know a commercial source for methyl lead
acetate?
thanks in advance,
Tommi
--
Tommi Kajander, Ph.D.
Macromolecular X-ray Crystallography
Research Program in Structural Biology and Biophysics
Institute of Biotechnology
PO box 65 (Street address: Viikinkaari 1, 4th floor
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