7.012 Fall 2003
Solutions to 7.012 Problem Set 3
Question 1
You have two pure-breeding colony of mice. Colony I mice have black fur and long tails,
Colony II mice have golden fur and short tails.
You cross mice from each of these colonies.
F
0
black fur and
long tails
X golden fur and
short tails
g1
F
1
Brown fur and
long tails
a) Predict genotypes for the mice shown in the cross above. Define your notation.
i) black fur and long tails: BB LL
ii) golden fur and short tails: B’B’ ll
iii) Brown fur and long tails: BB’ Ll
b) You mate a male and a female from the F
1
generation. Given your prediction in (a), what
genotypes and phenotypes do you see in the F
2
generation, and in what ratios?
BB’ Ll X BB’ Ll
BL Bl B’L B’l
BL BBLL
black fur and long
tails
BBLl
black fur and long
tails
BB’LL
brown fur and
long tails
BB’Ll
brown fur and
long tails
Bl BBLl
black fur and long
tails
BBll
black fur and short
tails
BB’Ll
brown fur and
long tails
BB’ll
brown fur and
short tails
B’L BB’LL
brown fur and
long tails
BB’Ll
brown fur and
long tails
B’B’LL
golden fur and
long tails
B’B’Ll
golden fur and
long tails
B’l BB’Ll
brown fur and
long tails
BB’ll
brown fur and
short tails
B’B’Ll
golden fur and
long tails
B’B’ll
golden fur and
short tails
MIT Biology Department
7.012: Introductory Biology - Fall 2004
Instructors: Professor Eric Lander, Professor Robert A. Weinberg, Dr. Claudette Gardel
7.012 Fall 2003
Question 1, continued
Your collegue has two other colonies of pure-breeding mice. Colony III mice have white fur
and long tails, Colony IV mice have white fur and short tails.
You cross mice from each of these colonies.
white fur and
long tails
X white fur and
short tails
g1
Black fur and
long tails
c) How can you explain this result?
There are mutations in two different genes, F and W that result in the same recessive phenotype, white
fur. The cross could be:
ffWWLL (white fur with long tail) X FFwwll (white fur with short tail) to give:
fFWwLl = black fur with long tails
Question 2
In a hypothetical type of yeast, the biosynthetic pathway for phenylalanine (shown below) has
five reaction steps each catalyzed by a different enzyme (1 – 5). The pathway is known to
begin with phosphoenolpyruvate (PEP) and proceed via 4 intermediates W, X, Y, and Z to
phenylalanine.
PEP W X Y Z phenylalanine
1234 5
You want to identify the enzymes (five total) involved in this pathway by isolating yeast that
fail to synthesize phenylalanine (these yeast are referred to as “phe
-
”). You know that mutant
yeast that fail to synthesize phenylalanine (and thus can not grow without addition of
phenylalanine) are likely to be defective in one of the enzymes involved in the phenylalanine
synthesis pathway. You start with a population of wild-type (“phe
+
”) yeast, mutagenize it
with UV light, and allow the treated cells to grow into isolated colonies on plate 1 (see FIGURE
1). You then use the replica plating technique to transfer some yeast from each colony onto
plates 2, 3, 4, and 5. The contents of the growth medium are listed below each plate. Rich
medium contains all nutrients and allows growth of both wild type, and mutant cells.
Minimal medium contains nutrients sufficient to allow only wild-type, protoptrophic yeast to
grow. It will not support the growth of auxotrophic cells.
7.012 Fall 2003
FIGURE 1:
A
B
C
D
E
F
G
H
X
Y
A
F
A
B
F
AC
E
F
G
H
Y
A
B
C
D
E
F
G
H
X
Y
plate 1
plate 2
plate 3
plate 4
plate 5
rich medium
minimal medium + phe
minimal medium
minimal medium + PEP
rich medium
a) Plate 1 is the original rich medium plate that the mutagenized cells were grown on. It is
standard practice for the last plate in a series of replica plates to have the same growth
medium as the original plate. What purpose might this serve?
It is a control. You want to make sure that cells from each colony were transferred to all previous plates
so you can assess growth versus no growth.
b) You obtain some phe
-
colonies in this manner. Identify the colonies from FIGURE 1 that are
phe
-
C,G,E,H,Y
c) You notice that some colonies do not grow on plates containing minimal medium +
phenylalanine (plate 2). Identify these colonies and give one possible explanation for the
growth behavior of these colonies.
Cells from colonies B, D, and X may have a mutation in a gene that is important for the synthesis of any
compound other than phenylalanine.
d) This strategy for isolating phe
-
mutants works well so you repeat the mutagenesis and
replica plating experiment to isolate more phe
-
mutants. You then perform a
complementation test on these phe
-
mutants.
i) What is a complementation test?
A complementation test consists of creating a diploid that carries two independently isolated
mutations and examining if the diploid has a mutant or a wildtype phenotype.
If the diploid has a wildtype phenotype, then one assumes that the two mutations are in different
genes. If the diploid has a mutant phenotype, then one assumes that the mutations are in the
same gene.
ii) What is the purpose of a complementation test?
A complementation test can identify how many different genes are represented in a group of
mutants.
7.012 Fall 2003
Question 2, continued
In the table below, a (+) indicates that the diploid created grows on minimal media, a (-)
indicates that the diploid fails to grow on minimal media.
m1 m2 m3 m4 m5 m6 m7 m8 m9 m10
m1- - ++++- +++
2- - -
m3++- ++++ +++
4+++- +++ ++-
m5++++- ++ +- +
6+++++- + -+
m7- - ++++- +++
8+++++- + -++
m9++++- ++ +-
10+++- +++ ++-
ii) Assign the mutants 1-10 into complementation groups.
m1, m2,m7
m3
m4,m10
m5, m9
m6, m8
e) You also characterize your mutants based upon which of the intermediates accumulates
m2: accumulates X
m3: accumulates Z
m4: accumulates PEP
m5: accumulates Y
m6: accumulates W
Based on the above data, you predict that
i) m1 has a mutation in gene___3___
ii) m2 has a mutation in gene___3___
iii) m3 has a mutation in gene___5___
iv) m4 has a mutation in gene___1___
v) m5 has a mutation in gene___4___
7.012 Fall 2003
Question 3
Replica plating has been used to address profoundly important questions in bacterial genetics.
For example, in the 1940's there was much debate regarding the issue of whether or not
mutants pre-exist in a population of bacteria. Researchers observed that when they inoculated
wild type (pen
S
) bacteria onto growth medium containing penicillin, and thus selected for
bacteria that had mutated to become penicillin resistant, a small fraction (~10
-6
) of cells would
always grow. Thus, pen
R
colonies had arisen from a pen
S
population. There were two models
for this:
Model A: "Directed Mutations" One group of researchers argued that these mutants originated
as a result of the selective pressure. Their line of reasoning was that the bacteria can sense the
need to grow on penicillin and that a small fraction of them successfully mutate in a directed
manner so that they become pen
R
.
Model B: "Pre-existing Mutations" A second group of researchers argued that pen
R
mutants
pre-existed within the wild type population before ever coming into contact with penicillin;
thus, (they argued) penicillin doesn't direct mutations, it simply reveals mutants.
Replica plating provided a rapid means for testing these two hypotheses. The following is a
simplified version of the experiment. Plate 1 contains a "lawn" of cells (a solid layer of cells
packed together), all of which are the offspring of a single, wild type cell. About 5 X 10
6
cells
were spread on a plate, and after a day of growth, they formed a lawn containing about 10
9
cells. Plate 1 was used as the master plate that was replicated onto plates 2, 3, 4, and 5.
The distribution of colonies on plates 3, 4, and 5 is identical.
a) Which of the two hypotheses (directed mutations or pre-existing mutations) does this result
more strongly support. Explain your reasoning.
These data support Model B, the pre-existing mutations model. Each pen
R
colony on plate 3 is also
represented on plates 4 and 5, suggesting that these pen
R
colonies already existed on plate 1. If the
mutations were arising anew upon exposure to penicillin, you would expect different patterns of pen
R
colonies on plates 3, 4, and 5.
7.012 Fall 2003
Question 4
Shown below is a diagram of a replication fork in a double-stranded (ds) DNA molecule found
in a prokaryotic cell. Each DNA strand (A and B) serves as a template for polymerization by
DNA polymerase, resulting in the formation of a newly synthesized "daughter" DNA strand.
Replication fork
moves in this
direction
5’
3’
3’
5’
strand A
strand B
a)
i) On which template strand (A or B) would there be continuous replication by DNA
polymerase? What is this newly synthesized daughter strand called during DNA
replication?
Strand A will be copied in a continuous fashion. The daughter strand will be the leading strand.
ii) On which template strand (A or B) would there be discontinous replication by DNA
polymerase? What is this newly synthesized daughter strand called during DNA
replication?
Strand B will be copied in a discontinuous fashion. The daughter strand will be the lagging
strand.
iii) Chemicals that inhibit the enzyme DNA ligase will primarily affect synthesis on one
of the two template strands (A or B). Explain on which template strand (A or B)
polymerization will be primarily affected and why this occurs.
Synthesis of the lagging strand using strand B as a template will be affected most by inhibition of
DNA ligase. Without DNA ligase, the Okazaki fragment can not be joined together to form a
contiguous length of DNA.
b) There are inaccuracies in the DNA molecule shown below.
g1g1g1 1 5 10
g1g1g15' A G T C C G A U G C 3'
| | | | | | | | | |
g1g1g15' T C A G G C T A T G 3'
i) Name three things that are wrong in the above DNA sequence.
7.012 Fall 2003
? The strand are not anti-parallel
? In DNA there should no be any U’s
? G would not base-pair with T
ii) What type of chemical interaction is indicated by a "
|
" in the above diagram? What
happens to these interactions during DNA replication?
This line indicates hydrogen bonding between the two complementary bases. It would represent
2 hydrogen bonds between A and T or 3 hydrogen bonds between G and C. these bonds are
disrupted to allow replication of the DNA and new bonds form with the newly synthesized
strands.
c) Shown below is the structure of a monomer used in nucleic acid synthesis.
g1g2
g3
OH
HH
O
CH
2
OPOPOP
HO
N
N
N
N
NH
2
OOO
HH
O
–
O
–
O
–
O
–
i) Would this monomer be used to form part of an RNA strand or a DNA strand?
Briefly explain your answer.
RNA because it has a 2’ OH
ii) In nucleic acid synthesis, one of the phosphate groups of this monomer is covalently
linked to a new strand that is being elongated. In the figure above, draw a circle around
the phosphate group that would be linked.
iii) When this monomer is already part of the newly synthesized strand, one of the
hydroxyl groups of this monomer will be linked to the phosphate group of the next
monomer added. In the figure above, draw a box around the hydroxyl group that will
be linked.