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packback 10-12

Does λ phage go to lytic or lysogenic pathway in the following conditions?

a) the λ phage encodes a nonfunctional Cro protein

b) the λ phage encodes a nonfunctional N or Q protein

c) the λ phage encodes a nonfunctional CI protein

d) the λ phage encodes a nonfunctional CII protein

e) the λ phage encodes a nonfunctional CIII protein

Background (Quick + Helpful for Understanding):

λ phage chooses between:

Lytic cycle = kill host, make new phage
Lysogenic cycle = integrate into host genome, stay dormant

Key regulatory proteins:

- Cro: Lytic Blocks CI expression

- CI (λ repressor): Lysogenic Represses lytic genes & maintains lysogeny

- CII: Lysogenic Turns on CI (and thus lysogeny) early after infection

- CIII: Lysogenic Protects CII from degradation

- N & Q: Lytic (anti-termination)Allow expression of lytic regulatory genes

a) Nonfunctional Cro Cro normally inhibits CI.
If Cro doesn’t work → CI wins → lysogeny established.

Can you explain the mechanism of DNA sequencing using dideoxy method and read the DNA sequence from a sequencing gel?

How the Dideoxy (Sanger) Method Works Key Idea

DNA polymerase builds DNA by adding nucleotides to a growing chain.
Normal nucleotide: dNTP → has a 3’ OH → chain continues
Dideoxynucleotide: ddNTP → no 3’ OH → chain stops when added

Step-by-Step Mechanism

Denature template DNA into single strands
Add:
- DNA primer (binds to known sequence)
- DNA polymerase
- All 4 dNTPs
- Small amount of ddNTPs (each labeled, historically radioactive or fluorescent)
DNA polymerase copies template
Whenever a ddNTP is incorporated → chain terminates
This produces many DNA fragments of different lengths, each ending at a specific base

How We Read it

The fragments are separated by size using gel electrophoresis

Shorter fragments travel further down
Each lane represents one nucleotide (A, T, G, C) if using a 4-lane gel (modern methods combine lanes with fluorescent bases, but same logic applies)

You read the gel:

Bottom → Top
because smallest fragment (lowest band) = earliest termination = first base after primer

So you read which lane each band is in:

Bottom → Top might read:
G → A → C → T → A → T → G …

To help you understand DNA sequencing, can you do the following?

write down a random DNA sequence, presuming that you’ve already known the sequence of the first 5 nucleotides.

a) Design the sequencing primer

b) Perform a virtual sequencing experiment

c) run the DNA products virtually on a gel

d) read the DNA sequence from your gel

Step 0 – Make up a DNA sequence (first 5 bases known)

Let’s say the strand we want to know is:

5'-ATGCC TAGACTGT-3'

We are told we already know the first 5 nucleotides:

Known: 5'-ATGCC-3'
Unknown (what we’ll sequence): TAGACTGT

So the unknown part we’ll “discover” by Sanger is:

5'-TAGACTGT-3'

a) Design the sequencing primer

We design a primer that binds just before the unknown region, i.e., to the known sequence ATGCC.

To keep it simple, we’ll just use those 5 known bases as the primer:

Primer (5'→3') = 5'-ATGCC-3'

Conceptually:

The template strand in the tube is the complement of our target strand.
Our primer binds to this complement and DNA polymerase extends it into the unknown region.

You don’t have to stress the template strand sequence for this question; the key is:
primer = known sequence at the 5' end of what we’re sequencing.

b) Perform a “virtual” Sanger sequencing experiment

We set up 4 reactions (classic version), each with:

Template DNA
Primer: 5'-ATGCC-3'
DNA polymerase
All 4 normal dNTPs
A small amount of one ddNTP in each tube:
- Tube 1: ddATP
- Tube 2: ddTTP
- Tube 3: ddGTP
- Tube 4: ddCTP

As DNA polymerase extends from the primer into the unknown region (TAGACTGT), sometimes it adds a normal dNTP and keeps going, and sometimes it accidentally adds a ddNTP, which stops the chain at that base.

Our newly synthesized unknown region is:

5'-TAGACTGT-3'
index the bases:
1: T
2: A
3: G
4: A
5: C
6: T
7: G
8: T

Where can termination occur?

ddTTP (T): positions 1, 6, 8 → fragments of length 1, 6, 8
ddATP (A): positions 2, 4 → fragments of length 2, 4
ddGTP (G): positions 3, 7 → fragments of length 3, 7
ddCTP (C): position 5 → fragment of length 5

(Remember: these lengths are for the newly added region after the primer.)

c) Run the DNA products “virtually” on a gel

We run the 4 reactions in 4 lanes on a polyacrylamide gel.

Let’s order the lanes (left → right) as:

Lane G | Lane A | Lane T | Lane C

Shorter fragments run farther (toward the bottom), longer fragments stay higher.

Using the fragment lengths we listed, here’s what the gel would look like conceptually:

Lane G (ddGTP): bands at lengths 3, 7
Lane A (ddATP): bands at lengths 2, 4
Lane T (ddTTP): bands at lengths 1, 6, 8
Lane C (ddCTP): band at length 5

Now, imagine the gel:

(top, largest fragments)

len 8: G | A | T● | C (T at position 8)
len 7: G●| A | T | C (G at position 7)
len 6: G | A | T● | C (T at position 6)
len 5: G | A | T | C● (C at position 5)
len 4: G | A●| T | C (A at position 4)
len 3: G●| A | T | C (G at position 3)
len 2: G | A●| T | C (A at position 2)
len 1: G | A | T● | C (T at position 1)

(bottom, smallest fragments)

You don’t need the exact picture on the exam, but you need to know:

Bottom = smallest fragment = first base after the primer
Each band tells you: “at this length, the chain ends in the base in this lane.”

d) Read the DNA sequence from the gel

To read the sequence:

Look at the bottom band first (shortest fragment = first base added after the primer).
Move upwards, noting which lane each band is in.
Write down the corresponding base.

From the “gel” above, going bottom → top:

len1 → T lane → T
len2 → A lane → A
len3 → G lane → G
len4 → A lane → A
len5 → C lane → C
len6 → T lane → T
len7 → G lane → G
len8 → T lane → T

So the newly synthesized unknown sequence is:

5'-TAGACTGT-3'

Put it together with the known first 5 nucleotides (ATGCC):

Full sequenced strand: 5'-ATGCCTAGACTGT-3'

That matches the “random” sequence we started with.