You plan to clone exon 11 of the HEXA gene (Section C) into the multiple cloning site (MCS) of the plasmid vector pUC19 illustrated below. You PCR amplify only the 184 bp DNA region representing exon 11 of HEXA from human DNA as a blunt-ended dsDNA fragment, and purify the amplicon. Next you digest the vector pUC19 with the restriction enzyme (RE) Smal to obtain linear plasmid DNA. You mix the PCR product and linear plasmid, add some DNA ligase enzyme in an appropriate buffer, and incubate overnight at 16°C. The ligation mixture is used to transform competent E. coli cells, which are subsequently streaked out onto agar plates containing ampicillin, X-gal and IPTG. HEXA exon 11 sequence: attcagccagacacaatcatacaggtgtggcgagaggatattccagtgaactatatgaaggagctggaactggtc accaaggccggcttccgggcccttctctctgccccctggtacctgaaccgtatatcctatggccctgactggaag gatttctacatagtggaacccctggcatttgaag PUC 19 plasmid map: 2686 1 Amp 0 lacZ EcoRI (390) Smal (410) BamHI (420) MCS Kpnl (430) LacR binding site Plac Pstl (440) PUC19 2686 bps PMB1 ori Complete the table below by providing the recognition sequences, cleavage positions and types of termini generated for the following three restriction enzymes which cut in the MCS of pUC 19; also indicate the number and position of cut sites for each enzyme in the 184 bp exon 11 amplicon. Enzyme Recognition sequence and Type of termini Number and position of cut sites in exon 11 cleavage position SmaI BamHI KpnI

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You plan to clone exon 11 of the HEXA gene (Section C) into the multiple cloning site (MCS) of the
plasmid vector pUC19 illustrated below. You PCR amplify only the 184 bp DNA region representing
exon 11 of HEXA from human DNA as a blunt-ended dsDNA fragment, and purify the amplicon.
Next you digest the vector pUC19 with the restriction enzyme (RE) Smal to obtain linear plasmid
DNA. You mix the PCR product and linear plasmid, add some DNA ligase enzyme in an appropriate
buffer, and incubate overnight at 16°C. The ligation mixture is used to transform competent E. coli
cells, which are subsequently streaked out onto agar plates containing ampicillin, X-gal and IPTG.
HEXA exon 11 sequence:
attcagccagacacaatcatacaggtgtggcgagaggatattccagtgaactatatgaaggagctggaactggtc
accaaggccggcttccgggcccttctctctgccccctggtacctgaaccgtatatcctatggccctgactggaag
gatttctacatagtggaacccctggcatttgaag
PUC 19 plasmid map:
2686 1
Amp
0
lacZ
EcoRI (390)
Smal (410)
BamHI (420)
MCS
Kpnl (430)
LacR binding site
Plac
Pstl (440)
PUC19
2686 bps
PMB1 ori
Transcribed Image Text:You plan to clone exon 11 of the HEXA gene (Section C) into the multiple cloning site (MCS) of the plasmid vector pUC19 illustrated below. You PCR amplify only the 184 bp DNA region representing exon 11 of HEXA from human DNA as a blunt-ended dsDNA fragment, and purify the amplicon. Next you digest the vector pUC19 with the restriction enzyme (RE) Smal to obtain linear plasmid DNA. You mix the PCR product and linear plasmid, add some DNA ligase enzyme in an appropriate buffer, and incubate overnight at 16°C. The ligation mixture is used to transform competent E. coli cells, which are subsequently streaked out onto agar plates containing ampicillin, X-gal and IPTG. HEXA exon 11 sequence: attcagccagacacaatcatacaggtgtggcgagaggatattccagtgaactatatgaaggagctggaactggtc accaaggccggcttccgggcccttctctctgccccctggtacctgaaccgtatatcctatggccctgactggaag gatttctacatagtggaacccctggcatttgaag PUC 19 plasmid map: 2686 1 Amp 0 lacZ EcoRI (390) Smal (410) BamHI (420) MCS Kpnl (430) LacR binding site Plac Pstl (440) PUC19 2686 bps PMB1 ori
Complete the table below by providing the recognition sequences, cleavage positions and types
of termini generated for the following three restriction enzymes which cut in the MCS of pUC
19; also indicate the number and position of cut sites for each enzyme in the 184 bp exon 11
amplicon.
Enzyme
Recognition
sequence and
Type of termini
Number and position
of cut sites in exon 11
cleavage
position
SmaI
BamHI
KpnI
Transcribed Image Text:Complete the table below by providing the recognition sequences, cleavage positions and types of termini generated for the following three restriction enzymes which cut in the MCS of pUC 19; also indicate the number and position of cut sites for each enzyme in the 184 bp exon 11 amplicon. Enzyme Recognition sequence and Type of termini Number and position of cut sites in exon 11 cleavage position SmaI BamHI KpnI
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