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bGH poly(A) signal (6977 6993) M13 Reverse PCDNA3.1- 9202 bp (6939) BstZ171 (6898 . 6917) EBV-rev (6887) Bsml (6844 6863) SV40PA-R (6649) BstBI (6503 6522) Neo-F (6483) Rsril SV40 ori (6364) BSSHII SV40 promoter PpuMI (3289) (5893 5912) Neo-R fl ori (5780) Smal (5778) TspMH - Xmal (5757) Avrll (5756) Stul 14000 15000 (5685. 5704) SV40pro-F BbvCI (3798) (5438 5458) PBABE 3 (5298 5319) Flori-F (5088 . 5107) Flori-R (4725 4742) BGH-rev (4709) Pmel (4704) Apal (4700) PSPOMI PaeR71 PspXI Xhol (4688) Xbal (4694) 13000 M13 rev d bej | signal R/KanR 6000

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QUESTION 2 The SARS-COV-2 pandemic resulted in the desire to design ELISA assays to either detect antibodies against SARS-CoV-2 protein (previous infection), or detect viral protein (current infection). You plan to express the mutant spike protein variant using the plasmid pictured below as your template. Here's the sequence you want to put in its place: https://www.ncbi.nlm.nih.gov/nuccore/AY429073.1?report=fasta, this is the DNA sequence you're going to buy as a gene block! But you need to add a couple things to it first so it'll get into the plasmid. To do so, you're going to need to remove the current insert (represented by the yellow arrow beginning at position 833-4867). Question: What restriction sites are you going to add at the ends of the gene? Answer can be in nucleotides or the enzyme name. For the first blank fill in the site name/sequence you'd add at the beginning of the gene (5' / C-terminus end) and for the second blank fill in the sequence/site name you'd add at the end of the gene (N- terminus end). (9178 .. 9197) pRS-marker Nrul (140) (9132) SgrDI (9015) Sspl Mlul (160) Spel (181) Ndel (416) SnaBI (522) (8761 .. 8780) Amp-R (8581) Pvul CMV-F (701 .. 721) Eco53kl (748) Sacl (750) 9000 T7 (795.. 814) Nhel (827) Bmtl (831) BsmBI (873) CMV en... 1000 CMV promoter T7 promoter 747R1RD322oriF 10008