#!/bin/csh # # set CCP4 and SOLVETMPDIR variables: # setenv CCP4_OPEN UNKNOWN setenv SOLVETMPDIR /var/tmp setenv SYMINFO /usr/local/lib/solve/syminfo.lib setenv SYMOP /usr/local/lib/solve/symop.lib # # solve_giant < solve.log !command file to read in raw MAD data, scale, analyze and solve it---- title armadillo repeat of beta catenin 4-wavelength MAD data logfile mad.logfile ! write out most information to this file. ! summary info will be written to "solve.prt" @solve.setup ! get our standard information read in readformatted ! or: readdenzo, readtrek, readccp4_unmerged unmerged ! or; premerged mad_atom se refscattfactors ! do not refine scattering factors (you can if ! you want though) ! Comment out next line if you don't know any sites checksolve ! compare solutions to the one input below lambda 1 ! info on wavelength #1 follows label Wavelength # 1 ! a label for this wavelength rawmadfile l1.int wavelength 0.9000 ! wavelength value fprimv_mad -1.6 ! f' value at this wavelength fprprv_mad 3.4 ! f" value at this wavelength ! list of all SE positions in refined beta-catenin ! structure (offset by 0.5 in y from PDB file) atomname se xyz 0.2631041 0.6633824 2.8978506E-02 xyz 0.4166300 0.6113137 7.7325497E-03 xyz 0.4765674 0.7249608 2.5320712E-02 xyz 0.4591554 0.7427059 0.4719517 xyz 0.4083922 0.7455686 0.1403100 xyz 0.4416372 0.8393628 7.6342024E-02 xyz 0.1327285 0.4970000 0.4364171 xyz 9.6379094E-02 0.5855882 0.3802352 xyz 7.6066948E-02 0.6245000 0.3974865 xyz 0.1150683 0.7795883 0.3715025 xyz 0.1385160 0.7238529 0.4098982 xyz 9.2073016E-02 0.7063529 0.4022779 xyz 0.2152710 0.8265882 0.3764597 xyz 0.3304202 0.6161765 0.2311389 xyz 0.1806852 0.8512745 0.1618233 lambda 2 rawmadfile l2.int wavelength 0.9794 fprimv_mad -11.44 fprprv_mad 8.74 lambda 3 rawmadfile l3.int wavelength 0.9797 fprimv_mad -12.83 fprprv_mad 2.56 lambda 4 rawmadfile l4.int wavelength 0.9897 fprimv_mad -2.42 fprprv_mad 1.13 nres 700 [approx # of residues in protein molecule] nanomalous 15 [approx # of anomalously scattering atoms per protein] acceptance 0.10 SCALE_MAD ! read in and localscale the data ANALYZE_MAD ! run MADMRG and MADBST and analyze all the Pattersons SOLVE ! Solve the structure EOD # # Now run Resolve to do density modification # (You can download it from http://resolve.lanl.gov # if you do not have it yet) # resolve_giant << EOD > resolve.log !solvent_content 0.40 ! solvent fraction seq_file weis.seq compare_file coords_met.pdb EOD # # That's it! Now resolve.mtz has your updated phases # echo 'Here are your SOLVE and resolve files:' # ls -l solve.prt solve.mtz solve.ezd resolve.mtz # echo 'All done.'