User:Nzimm
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Neil Zimmerman
Bio
- MIT Class of 2009
- Major: Biological Engineering
- Minors: Management and Music
- Varsity Soccer
- Wind Ensemble (Clarinet)
20.109
M13K07 Genome Engineering Plans:
| Gene | Plans |
|---|---|
| I | Change # of protein copies expressed to experiment with different sized channels |
| II | Modify residues to allow deactivation of p2 under certain conditions so that replication of + strand can be regulated |
| III | Insert myc to allow detection with an antibody |
| IV | Change # of protein copies expressed to experiment with different sized channels |
| V | Add fluorescent tag to monitor levels of p5-ssDNA complex |
| VI | Modify residues to help p3 bind more effectively to the ToIA protein on the E. coli F pilus |
| VII | Minimize the bulk of the protein to allow more room for modifications on p9 |
| VIII | Insert myc (as in III) or another tag to serve as a “hook” for attaching constructs to M13 |
| IX | Add residues to N-terminus to present on the outside of the phage coat |
| X | Add sensitivity to different stimulus than that of p2 in order to regulate replication of + strand in another fashion |
| XI | Modify residues to allow proteins other than p8 to embed in the membrane and serve as the phage filament coat |
M13K07 Genome Refactoring:
In refactoring the M13K07 genome between the HpaI site in gene II and the BamHI site in gene III, I separated all overlapping elements across the region by copying overlapping sequences and placing the elements adjacent to one another on the refactored sequence. As a result, the refactored region is 1,000 bp larger than the original sequence. I also added annotation for & refactored the open reading frames of genes 2, 5, 7, and 10, which are not annotated in the M1307 part in the registry. I inserted the sequence encoding the myc protein into g3. I intend to separate each element with two unique restriction sites, so that the elements can be isolated & manipulated more easily. I initially proposed to add a fluorescent tag like GFP to g5, but seeing as how GFP is nearly 3 times the size of the protein product of g5, I chose to leave g5 unaltered. Below is a table describing the overlaps that were refactored.
| Overlapping elements | Action |
|---|---|
| rbs g7 & g5 ORF | copied overlapping sequence & placed rbs g7 adjacent to the 3' end of the g5 ORF |
| promoter g8 & rbs g9 | copied overlapping sequence & placed rbs g9 adjacent to the 3' end of promoter g8 |
| promoter g3 & g8 ORF | copied overlapping sqeuence & placed promoter g3 adjacent to the 3' end of g8 ORF |
| g10 ORF, g10 rbs, g10 promoter, g5 promoter, & g2 ORF | copied g2 ORF & placed adjacent to 5' end of other (non-overlapping) elements |
| inserted the sequence encoding the myc protein into the BamHI site of g3 |
Current Courses
Other
Email: nzimm (at) mit (dot) edu
SAGA subunits, S. cerevisiae
| Ada subunits | size,chromosome,null p-type | notes |
|---|---|---|
| Ada1 (aka HFI1, SUP110, SRM12, GAN1) | 1.467 kb/489 aa, Chr. XVI, viable |
"Histone H2A Functional Interactor"; Adapter protein involved in structural integrity of SAGA |
| Ada2 (aka SWI8) | 1.305 kb/434aa, Chr. IV, viable |
"transcriptional ADAptor"; Transcription coactivator |
| Ada3(aka NGG1, SWI7) | 2.109 kb/702aa, Chr. IV, viable |
Transcriptional regulator involved in glucose repression of Gal4p-regulated genes |
| Gcn5 (aka ADA4, SWI9) | 1.32 kb/439aa, Chr. VII, viable |
"General Control Nonderepressible"; Histone acetyltransferase, acetylates N-terminal lysines on histones H2B and H3; this is the catalytic subunit |
| Ada5 (aka SPT20) | 1.815 kb/604aa, Chr. XV, viable |
"SuPpressor of Ty"; involved in maintaining the integrity of the SAGA transcriptional regulatory complex |
| Spt subunits | size, chromosome, null p-type | notes |
|---|---|---|
| Spt3 | 1.014 kb/337aa, Chr. IV, viable |
interacts with Spt15p to activate transcription of some RNA polymerase II-dependent genes, also functions to inhibit transcription at some promoters |
| Spt7(aka GIT2) | 3.999 kb/1332aa, Chr. II, viable |
involved in proper assembly of the complex; also present as a C-terminally truncated form in the SLIK/SALSA transcriptional regulatory complex |
| Spt8 | 1.809 kb/602aa, Chr. XII, viable |
required for SAGA-mediated inhibition at some promoters; not present in SLIK/SALSA complex |
| Spt20 (aka Ada5) | 1.815 kb/604aa, Chr. XV, viable |
maintains integrity of complex |
| TAF subunits | size, chromosome, null p-type | notes |
|---|---|---|
| TAF5 (aka TAF90) | 2.397 kb/798aa, Chr. II, inviable | "TATA binding protein-Associated Factor"; RNA polymerase II transcription initiation and in chromatin modification (90 kDa subunit) |
| TAF6 (aka TAF60) | 1.551 kb/516aa, Chr. VII, inviable | 60 kDa subunit with same function as above; similar to Histone H4 |
| TAF9 (aka TAF17) | 0.474 kb/157aa, Chr. XIII, inviable | 17 kDa subunit; similar to Histone H3 |
| TAF10 (aka TAF23, TAF25) | 0.621 kb/206aa, Chr. IV, inviable | 145 kDa subunit |
| TAF12(aka TAF61, TAF68) | 1.620 kb/539aa, Chr. IV, inviable | 61/68 kDa subunit; similar to Histone H2A |
| Tra1 subunit | size, chromosome, null p-type | notes |
|---|---|---|
| Tra1 | 11.235 kb/3744aa, Chr. VIII, inviable | interacts with acidic activators (e.g., Gal4p) which leads to transcription activation; similar to human TRRAP, which is a cofactor for c-Myc mediated oncogenic transformation |
| other subunits | size, chromosome, null p-type | notes |
|---|---|---|
| Sgf73 | 1.974 kb/657aa, Chr. VII , viable |
"SaGa associated Factor"; formation of the preinitiation complex assembly at promoters (73 kDa subunit) |
| Sgf29 | 0.779 kb/259aa, Chr. III, viable |
29 kDa subunit of SAGA histone acetyltransferase complex |
| Sgf11 | 0.3 kb/99aa, Chr.XVI, viable |
Integral subunit of SAGA histone acetyltransferase complex, regulates transcription of a subset of SAGA-regulated genes, required for the Ubp8p association with SAGA and for H2B deubiquitylation (11 kDa) |
| Ubp8 | 1.416 kb/471aa, Chr. XIII, viable |
Ubiquitin-specific protease - required for SAGA-mediated deubiquitination of histone H2B |
| Sus1 | gene with intron, Chr. II, viable |
"Sl gene Upstream of ySa1"; involved in mRNA export and interacts with the SAGA histone acetylase complex for transcription activation; component of the SAGA histone acetylase complex; high concentrations at nuclear pores |
