Title: Twohybrid approaches to finding proteinprotein interactions
1Two-hybrid approaches to finding protein-protein
interactions
Yeast two-hybrid -based on the fact that
transcription factors such as yeast GAL4 have
independently operating transcriptional
activation and DNA-binding domains that can
be separated from each other -bait protein is
fused to a DNA-binding domain (BD) and screened
against a cDNA library in which cDNAs
are expressed as fusion proteins with an
activation domain (AD) -when binding occurs
between bait and library protein, a
functional transcription factor is formed
that can turn on reporter genes with
the appropriate target sequences in
their promoter-enhancer region -activation
domains used in yeast two-hybrid
screening -GAL4 -viral protein VP16 -acidic
bacterial peptide B42
2-several variations of the yeast two-hybrid
system have been developed, in the lab we will be
using the interaction trap method -in this
system, the bait protein is fused to the BD of
the bacterial repressor LexA, while the library
proteins are fused to AD of B42 -reporter genes
contain LexA operator sequences and will be
turned on by the chimaeric GAL4-LexA factor when
protein-protein interactions occur between bait
and library -yeast host strain in this system is
EGY48 which has the genotype a, his3, trp1,
ura3-52, lex(leu2)3a -bait is cloned into
pEG202 where it is fused to BD of LexA -pEG202
is selected for by growth on his-
medium -library is cloned into pJG4-5 where
cDNAs can be expressed fused to B42 -pJG4-5 is
selected for by growth on trp- medium
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4-numerous cDNA libraries have been created that
will work in the interaction trap system -lacZ
reporter gene under control of lexA operator is
present in plasmid pSH18, which is selected for
by growth on ura- media -two-hybrid
interactions are detected through the expression
of the two reporter genes leu2 and
lacZ -expression of leu2 is selected for by
growth on leu- medium, while lacZ is detected
by growth on X-gal
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6Variations on the yeast two-hybrid
technique Three-hybrid method for detecting
RNA-protein interactions - two-hybrid-derived
method has been developed that allows screening
for proteins interacting with a given RNA -this
system is commercially available from Invitrogen
as the RNA-Protein Hybrid Hunter kit -in this
system, the lexA BD is expressed as a fusion
with the coat protein of the MS2 bacteriophage
using the vector pHybLex/Zeo- MS2 -the RNA of
interest (i.e. the bait RNA) is expressed as a
fusion with MS2 RNA by cloning the DNA encoding
it into the vector pRH3 or pRH5 -finally, the
cDNAs encoding the potential prey proteins are
included in a vector that will express them as
fusions with an AD, for example that from VP16 or
B42 -all 3 vectors are introduced into the
L40-ura3 strain of S. cerevisiae and tested for
reporter gene expression
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8-in this system the lexA operator-containing
reporter genes are HIS3 and lacZ -system is
based on the observation that the MS2 coat
protein binds to the MS2 RNA with high
specificity at a 33 nucleotide sequence that
forms a hairpin loop structure -reporter gene
expression is induced by joining the lexA BD to
the AD through a three-hybrid connector
consisting of (i) MS2 coat protein (ii)
MS2/bait RNA (iii) RNA-binding prey protein
9-efficacy of this method has been tested by
looking at two well known RNA-protein
interactions -recall that the iron response
element (IRE) is a stem-loop structure found in
the untranslated regions of mRNAs encoding
certain proteins involved in iron
utilization -for example, the protein
transferrin is involved in transporting iron into
the cell when cytoplasmic iron levels are high,
transferrin levels are low -this responsiveness
is controlled at the level of mRNA
stability -transferrin mRNA has IREs in its 3
UTR -when iron levels are low, an IRE
binding protein (IRP) binds to IREs in the
transferrin mRNA, probably by inhibiting the
function of destabilizing elements in the
vicinity -thus, when iron is low the transferrin
mRNA is stable and translated -when iron levels
are high, iron binds to IRP which then
dissociates from transferrin mRNA, exposing the
destabilizing elements and promoting degradation
10-tests with IRE and IRP demonstrate that lacZ
expression is only induced when all components of
the three-hybrid are present
11-another RNA-protein interaction used to test
the system is binding of the HIV Tat
transcription factor to the target TAR sequence
in the RNA product of a previous round of
transcription
12One-hybrid identification of DNA-protein
interactions -if one has a short DNA sequence
that is suspected to be a protein binding site, a
one-hybrid screen can be done -in this system,
the DNA sequence of interest (bait) is inserted
upstream of the minimal promoter of the reporter
gene as multiple tandem copies -cDNA library is,
as usual, expressed as fusion to AD -if
expressed protein binds to bait DNA, this will
result in functional transcription factor and
reporter gene expression
13A three-hybrid approach to investigate
interactions involving three proteins -the
pBridge vector replaces the usual BD bait
vector -with pBridge, one protein is fused to BD
and constitutively expressed, but another protein
of interest is expressed only in the absence of
methionine (can be switched on and off) -the
other protein is expressed from a conventional
two-hybrid vector as a fusion to an AD -effects
of bridging protein on interaction between
other two proteins can be tested by comparing
reporter gene expression with or without
induction of the bridging protein
14The bridging protein can contribute to the
interaction between the other two proteins in a
number of ways -link two proteins together by
binding both -stabilize a weak interaction
between two proteins -modify one or both
of the proteins -inhibit the two-hybrid
interaction
15Two-hybrid analysis in bacteria - a bacterial
two-hybrid system has been developed, based on
the observation that an arbitrary interaction
between a DNA-bound protein and bacterial RNA
polymerase can activate transcription -such an
interaction stabilizes the binding of RNA
polymerase close to promoter, and probably
acts similarly to the UP element in strongly
expressed bacterial genes -in the BacterioMatch
system marketed by Stratagene, the bait protein
is expressed as a fusion with the cI l
repressor protein -the ampr and lacZ reporter
genes have an upstream l operator sequence that
will bind the cI-bait fusion -the target
proteins from cDNA library are expressed as
fusions with the a subunit of RNA polymerase -if
bait interacts with target, we will get linking
of DNA-bound cI with a subunit of RNA polymerase
and enhanced transcription due to stronger
association with promoter
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17AraC/LexA-based E. coli two-hybrid system -this
system based on the ara operon arabinose-
AraC protein acts as transcriptional activator
- arabinose- AraC causes DNA loop formation,
blocking access of RNA polymerase
18-the bait protein is fused to AraC, while the
prey is fused to LexA -in the absence of
interaction, reporter gene expression is turned
ON through AraC acting as an activator of
transcription -when there is interaction between
bait and prey, the promoter region is bent into
a repression loop, as the prey-LexA fusion
protein is also bound to LexA operator sequences
in the reporter gene promoter region -in this
system binding of bait to prey is
therefore visualized by REPRESSION of reporter
gene expression
19Mammalian two-hybrid assays -mammalian
two-hybrid analysis is generally used to validate
mammalian protein-protein interactions detected
in other systems -because the assay is
performed in mammalian cells, proteins are more
likely to be in a native confirmation and
experimental results are more likely to represent
biologically significant interactions -a kit
for doing mammalian two-hybrid is marketed by
Clontech -the reporter gene used is bacterial
chloramphenicol (CAM) acetyl transferase
(CAT) -CAT is one of the most heavily used
reporter genes used to measure eukaryotic
transcription -in one of the most popular CAT
assays , extracts from cells of interest are
mixed with radioactive CAM and an acetyl donor
(acetyl CoA) -thin layer chromatography is used
to separate CAM from its acetylated
products -the higher the promoter activity the
greater the concentration of acetylated
CAM -because eukaryotic cells lack endogenous
CAT, the background CAT level is zero
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22REFERENCES Finley, R. L., Jr., and Brent, R.
(1995). Interaction trap cloning with yeast. In
DNA Cloning, Expression Systems A Practical
Approach, B. D. Hames and D. M. Glover, eds.
(Oxford Oxford University Press), pp.
169-203. Golemis et al. Current Protocols in
Molecular Biology, Supplement 46. Interaction
Trap/Two-Hybrid System to Identify Interacting
Proteins. Wiley. Hu JC, Kornacker MG, Hochschild
A. Escherichia coli one- and two-hybrid systems
for the analysis and identification of
protein-protein interactions. Methods. 2000
Jan20(1)80-94. Lewin B. Genes VII . Oxford
University Press, 2000. SenGupta DJ, Zhang B,
Kraemer B, Pochart P, Fields S, Wickens M. A
three-hybrid system to detect RNA-protein
interactions in vivo. Proc Natl Acad Sci U S A.
1996 Aug 693(16)8496-501. Weaver, RF.
Molecular Biology. McGraw Hill,2002. Websites
http//www.clontech.com/ http//www.invitrogen.co
m/ http//www.stratagene.com/