MASARYK UMVB8TTY
Design of PCR Primers
gtča I lhj I i u I uuacuai (j ATCATGTTTT CCTTGATATC ATGT "GCTTCAACA CTCCAAATAC AGAGGTAATT AAATATTATT ATCA OATAATATG TTATTGATTT TTTGTTTGTG ATTTCATTTA GATTT "CTATGATTT CTTAGCATGA AATACAATTT ttgg AG AAA C AACT TTAAAAACA aaacttgaat TTTGAGAAAT TCAAAGATGT TATA" GTCAAAATT TAACAATTAT TCTTCTAAAT CATC CG G ATT CCGT BTACACATCT ACAATTTTCA ATTGAGGTAT TCTTGTTTTG ATGC 3ACGAATAGT TTGATTGATA AAAAAAATTC TAACCAATAT G ATA jTTTATTTTC I I M TGTCAA ACCATACTTT ATACTATGTA AC^TT BAGATTATTG AAAATAGTTT ATTTATAAAA TAGTAACCTA TTGT1 \AAAAAAAAA AAAAAATTGT AAATCGTGTT TGCAAACGAC ATG1 'CTTAGTTTJK AAACTVgcTg ATaTTcTFCA AATCGACTGT TCTT, ^ATCAACCflA ttaooatoaa t oa oaa*mAA TTGTAAACAC TTCA VTGGTGATTT TAAAGAATAT GTTTTACTTA TGTTATGAAC TATC" TGTGAAATA TTTCATAACT AATGTGGAAA ACTATATAAC CCCT VAAACGTAAG TAAAATTTAT GAAATCCTAT CATTTTTAAA GGTT> VTCAAAAAGT AATAATTCTT GGTACTTGCA ATAT I I I I GT CA1H7 "AGTTTATTA ATTTTATTTT GATTAAATGG TTTTAGATCC ATCAG íAGATCGCAG TTATAGCTGT AGACGATCCG AAGAAAGCAT TA1 AAAAATTCAA CGAGACAATA TAGATCTCAT AATCACAGAT TAT1 CTGGTATGAA CGGTTTACAA CTCAAAAAAC AAATCACTCA GGfi AATTTACCGG TCTTAG GTAA CAT I í I I I GT TCTTTACAAC TTAA
Proteomics Core Facility
CEITEC Central European Institute of Technology NCBR National Centre for Biomolecular Research
Hana Konečná
CG920 Genomics Lecture 12
OLIGONUCLEOTIDES
• definition
• aplications i
• modifications • design of sequence
• synthesis • rules
• purification • software OLIGO 7
• quality control • example
MASARYK
uiwBsrrv
oligonucleotide
short single stranded structure DNAor RNA (also PNA) hydroxyl on both ends (no phosphate on 5-end as usual)
orientation! polymerase
5' end H
|]TT| MASARYK
[lull uiwBsrrv
Aplications of synthetic oligonucleotides
• primers for synthesis of complementary DNA
PCR, Real-Time PCR
• gene synthesis and recombinant proteins
• hybridisation probes for cloning
• site directed mutagenesis
• sequencing ang genetic profiling
• diagnostics - tests and biosensors
• gene arrays
• blocation of gene expression antisense oligo
• prospective therapeutics and DNA vaccines
• NMR monitoring of DNA - protein interactions
• structural X-ray analysis of NA
4
MASMYK UMVBSTTY
• degeneration
• end of sequence
• bases
• phosphate
• carbohydrate
• PNA
[5J-conJugate|^
B heterocyclic base
phosphodiester bridge
B-o-deoxyribose       ' 0 (sugar)
0=P-o"
B
V
o
-conjugate
MASARYK
uiwBsrrv
Degenerated oligonucleotides
Examples:
ACG TAC GTA CGTACG TAC non-degenerated
ACG TAM GTA CGT ACG TAC       M = A/C
ACG TAC GTA CDT ACG TAC        D = A/G/T
ACG TAC GTA CGT ACG NAC        N = A/C/G/T
MASARYK
uiwBsrrv
Degenerated oligonucleotides
2-deoxyinosin
M	AorC
R	AorG
W	AorT
S	C orG
Y	C orT
K	G orT
V	AorC orG
H	AorC orT
D	AorG orT
B	C orG orT
N	G or A orT or C
X	G or A orT or C
MASARYK UMVBtSTTY
postsynthetic modifications
sequencing fragmenation analysis gene arrays Real-Time PCR
	Phosphorylation
-►	Amino group
-►	Thio group
	Digoxigenin
-►	Biotin
	Enzymes
	Psoralen
	Acridine
	Cholesterole
-►	Fluorescent dyes
	Quenchers
	2,4- dinitrophenyl
	Spacer
	Branching
	Blocation
MASARYK
uiwBsrrv
derivatized matrix
Phosphate Thio group Amino group Spacer Acridine Biotin
Fluorescent dyes Quenchers Cholesterole 2,4 dinitrophenyl
9
MASARYK
uiwBsrrv
rawwflRD pniMcn
• 2x labeled probe
• REPORTER
• QUENCHER
2, Strand displacement: When the probe is intact, the reporter dye emission is quenched.
r. a1
5_9,
r I'
3, Cleavage: During each extension cycle, the DNA polymerase cleaves the reporter dye from the probe.
SV J"
—^
B'
9'
4, Polymerization completed: Once separated from the quencher, the reporter dye emits its characteristic fluorescence.
MASARYK
uiwBsrrv
Other modifications
Phosphorothioates     <- backbone
Phosphorodithioates
H-phosphonates
Methylphosphonates
.... Modifications in 2'- position
carbohydrate-- modification
11
MASARYK UMVBtSTTY
TheraoeutiCS _* Nondegradable by nucleases!
Modification of phosphodiester
O 0 0
phosphorothioate        methylphosphonate phosphoramidate
S "CH2 "O
i I  2 i
CH2 H3C-N 0 = P-BH,
0 0 3-thioformacetal     methylene(methylimlnio) boranophosphate
12
MASARYK
UMVBsmr
ANTISENSE oligonucleotide
oligonucleotide or analogue complementary to segment of RNA or DNA inhibition of normal function due to coupling
Antigone (triplex) Ribozymo
Antisense
Sense/Aptamer
RNA with catalytic activity
13
MASARYK
uiwBsrrv
Peptidonucleic acid	PNA DNA
• uncharged molecule • binding with DNA/RNA N-(2-aminoethyl)-glycine-► i—NH 0 H2N—	N-terminal  """        ' \     ^ 5'-er^'^^ o=< o=p-o-RepeatJ     1     J \j L o=( o=p-o" 1     O       3 -end 0 C-terminal  °K 0=^-0" PNA DNA
14
MASARYK UIW9STTY
Peptidonucleic acid
noncharged molecule binding with DNA/RNA
N-(2-aminoethyl)-glycine-
•NH O
PH
R,N-
PNA
MASARYK
uiwBsrrv
Why PNA
• thermostable
• Tm not depending on salts
• high specificity
• high affinity
• resistant towards enzymes
Gambari R. Expert Opin Ther Pat. 2014, 24(3):267-94.
Peptide nucleic acids: a review on recent patents and technology transfer.
16
MASARYK UMVHWTTY
I
o=p-o
Locked Nucleic Acid I
• 2'-0, 4'-C methylene bridge
• supressed flexibility of ribofuranose ring
• structure is locked into rigid C3-endo conformation
• enhanced hybridisation
• outstanding biostability
Molecular Therapy (2012); 20 8, 1590-1598.
LNA-based Oligonucleotide Electrotransfer for miRNA Inhibition
MASARYK
uiwBsrrv
design synthesis
purification
EXPEDITE 8909
18
MASARYK UMVBWTY
Oligonucleotide Synthesis
synthesis on solid matrix from 3'-end to 5'-end anhydrous environment
O ii	B, O n
-O— P - o —, r t> n	II - 0— p _0 o- N
OH
Cleevage/Deprotection
^1
B,
°— P -O ^ J- I
I \ OR
Step 2. Coupling
^ O -
HO-
- o
Stepi. Deblocking
DMT- O
Activation	
E	ŕ
	- 0 — P - N(iPr),
	OR
♦ Tetrazole	
19
MASARYK
uiwBsmr
Quality Control
ISO.bia - 20.0U1
0.5
0.0
IS 20 Hln
25
30
35
HPLC perfusion chromatography
anex RP
20
MASARYK UMV9STTY
Perfusion chromatography
1341ong.bio - 20.0ul
classical sorbent
POROS
0.1JH
0,10-
0.05H
0.00
100
5     10    l's    20 ^2*5    30 35(^tg?
Min
134.bio - 20.0ul
2 6
: a ■
0.15H
0.1<H
0.05
0.004
	
	
---~J	v-,
0.0
2.5
Min
100
50
MASARYK UMV9STTY
Quality Control
Maldi-TOF MS CE
7 LOS
Mffl*/charge B
Capillary ckctoophocraü trace
MASARYK
uiwBsrrv
YIELD
Yield
85     85     75     75      65 65 crude purified crude purified crude purified
23
MASARYK UMVB8TTY
PURIFICATION
• Sephadex
• RP cartridge
• HPLC
ISO.big - 20.0131
MASARYK
uiwBsrrv
• manual
• computer assisted
www.protocol-online.org/prot/Research_Tools/Online_Tools/Oligo_Design/ind
Main features of good PCR primer sequence
• highly specific
• no dimers and hairpins
• stable duplexes with active sequence
• lightly unstable 3'-end
25
MASARVK UMV9STTY
OLIGO 6 • PCR primers
• hybridisation probes
• sequencing primers
OLIGO 7 (from 2008)
• TaqMan probes
• primers for nested PCR
• molecular beacons
• siRNA
26
MASARYK
uiwBsmr
Terminology of PCR primers
forward primer... part of the + string reverse primer... part of the - string
poi:     350      tm: 57.1
,,260,        , , 27Ü _        ,|2SÜ,        ,i^0,          , 300 _          , 31-Ü _        i,^IJi        _ , 330 _          , 340 _	3S0 ,
CCTCCCTCTCACTACTCA ►   ►   ►   ►   ►......►......►......►   ►   ►   ► i	hhhhhhthhth
	
TTAATGC CTG G CTGTGACTACTCACWtt EAAGGATGGTATTGAGC CTATGTG G G AAG A GAGAAAAACAAAC GGGGAGGAC GATG G CTAATTACATTGAACAAAGAffACACAGG AACH] ACC C	
AATTAC G GAC C GACACTGATGAGTGAAAAATTC CTAC CATAACTC G GATACAC C CTTCTACTC11111GTTTGCCCCTCCTGCTACCGATTAATGTA;	tCTTGTTTGTC GTCTCTG CTTCACTG GAG
	
	
LHPGCQY5   LFKO-G   IE   P   M   i   E   DE   KNKRGGRi        I   T L	NKQQRR5DL
UPPER - FORWARD - LEFT 5'-►
+ 5'-- 3'-
■ 3'
■ 5'
5'
LOWER - REVERSE - RIGHT
27
MASARYK UIW9STTY
Terminology
forward primer., reverse primer..
part of the + string part of the - string
pos:     350      tm: 57.1	
, 2E€ _          , 270 _        ,,230,           233             ^33             1-3             ^23             333 3^3	113 ÖG3
	
	
TTAATGC CTG G CTGTGACTACTCACI1111AAGGATGGTATTGAGCCTATGTGGGAAGATGAGAAAAACAAACGGGGmGGACGA GGCTAATTACATTGAACAAACAGCACACA«AAGTGACC C	
AATTAC GGACCGACACTGATGAGTGAAAAATTCCTAC CATAACTC GGATACACCCTTCTACTCTTTTTGTTTGCCCCTCCTGCTACC GATTAATGTAACTTGTTTGTCGTCTCTG CTTCACTG GAG	
.........ACTC G GATACAC CCTTCTACTC	
	
LMPGCDY5LFKDGIEPMWEDEKNKRGGRW ITL	NKQQRR5DL
UPPER - FORWARD - LEFT
5' » polymerase
+ 5] ^=^=| 3'
r I 15'
polymerase * 5'
LOWER - REVERSE - RIGHT
28
MASARYK UMVBtSTTY
Annealing of PCR primers
pos:
350
tm: 57.1
	, 2G0 _          , 29D _           300             1.3             12-1             33Ü 3^0	HO              100 170
		
		
TTAATG C CTG G CTGTGACTACTCAC t	111IAAGGATGGTATTGAGCCTATCTGGGAAGATGACAAAAACAAACGGGGAGGACGA GGCTAATTACATTGAACAAAtAGCAGAGACGAAGTGACC C	
AATTACGGACCGACACTGATGAGTGAAAAATTCCTAC CATAACTCGGATACACCCTTCTACTCTTTTTGTTTG C C C CTC CTG CTAC CGATTAATGTAACTTGTTTGTCGTCTCTG CTTCACTG GAG		
4                   4                   4                   1                   4 H	< ACTC G GATACAC CCTTCTACTC	
		
LMPGCDY5 L	F   K   D   G   I   E   P   M   W   E   DE   KNKRGGRW ITL	NKQQRR5DL
UPPER - FORWARD - LEFT
+ 5'-
————————————————————————— 3'
3'-5'
5' LOWER - REVERSE - RIGHT
29
MASARYK UMVHtSTY
5'CTTCTG CTCAATCTTTCTAC 3' FORWARD
+ ATGdCTTCTG CTCAATCTTT Cl"ACAACCAA AGCTCTGTCT TGAAAATCAA
^ 51 TGTCA i uu i i u i uuauua i u ATCATGTTTT CCTTGATATC ATGTCACGCA 101 TGCTTCAACA CTCCAAATAC AGAGGTAATT AAATATTATT ATCATATTAT 151 ATATAATATG TTATTGATTT TTTGTTTGTG ATTTCATTTA GATTTTTATT 201 TCTATGATTT CTTAGCATGA AATACAATTT TTGGAGAAAC AACTAGCAGT 251 TTTAAAAACA AAACTTGAAT TTTGAGAAAT TCAAAGATGT TATATATATA 301 TGTCAAAATT TAACAATTAT TCTTCTAAAT CATCCGGATT CCGTTTACAT 351 GTACACATCT ACAATTTTCA ATTGAGGTAT TCTTGTTTTG ATGCCTTTGA 401 GACGAATAGT TTGATTGATA AAAAAAATTC TAACCAATAT GATATATAAA 451 GTTTATTTTC TTTTTGTCAA ACCATACTTT ATACTATGTA ACTTTTTTAA 501 G AG ATT ATT G AAAATAGTTT ATTTATAAAA TAGTAACCTA TTGTTGAATT 551 aaaaaaaaaa aaaaaattgt aaatp.gtgtt TGCAAACGAC ATGTGATTTA 601 TCTTAGTTm AAACTAGCTG ATATTCTfCA AATCGACTGT TCTTATAAGT 651 AATCAACCÁA TTAQOATOAA TOAOAAÍAAA TTGTAAACAC TTCAATGAAA 701 ATGGTGATTT TAAAGAATAT GTTTTACTTA TGTTATGAAC TATCTCAAAT 751 TTGTGAAATA TTTCATAACT AATGTGGAAA ACTATATAAC CCCTCCATAC 801 AAAACGTAAG TAAAATTTAT GAAATCCTAT CATTTTTAAA GGTTAAACCA 851 ATCAAAAAGT AATAATTCTT GGTACTTGCA ATATTTTTGT CATTATATTT 901 TAGTTTATTA ATTTTATTTT GATTAAATGG TTTTAGATCC ATCAGTTATG 951 GAGATCGCAG TTATAGCTGT AGACGATCCG AAGAAAGCAT TATCTACTCT 1001 AAAAATTCAA CGAGACAATA TAGATCTCAT AATCACAGAT TATTATATGC 1051 CTGGTATGAA CGGTTTACAA CTCAAAAAAC AAATCACTCA GGAATTTGGA 1101 AATTTACCGG TCTTAGGTAA CATTTTTTGT TCTTTACAAC TTAAATTAAA
5' TGA AGA ATA TCA GCT AGT TT 3' REVERSE
MASARYK
uiwBsrrv
File: Human 4E.seq
Sequence
=1
DNA Sequence Sequence Length: Reading Frame: Current Oligo Length: Position:
		Selected Oligo	Position	Lcngtn		Feature	Location	
	B	Forward Primer	259	IS	) 1	source	-IS..1S5Ö-	
JJ		JLeierse Primer	32S			CD5	1..651	
JJ	B	Upper Oligo	—					
JJ	S	Lower Oligo	294	22				
JJ		PGR Product	S7nt					
1UOU        11 LOU
,13*0 .150U ,1L0!1
pos: I    350      tm: | 57,1
.........
,270 ,230 I I.........I I I I
,290 ,300 ,310 I.........ii~.......I I I I
,320
,330 ,340 I I I I.........I.......
350
,3E0 ,370 I.........I......
CC~CGC~C~CAC~AC~C^
TTAATG C CTG G CTGTCAtTAtTtAtTTTTTAAGGATGGTATTGAG C CTATGTG GGAAGATGAGAAAAACAAAC G G G GAG GAC GATG G CTJfTTTAC ATTG AAC
AATTACGGACCGACACTGATGAGTGAAAAATTC CTAC CATAACTCGGATACACCCTTCTACTCTTTTTGTTTG C C C CTC CTG CTAOJ^TTAATGTAACTTGTTTGTC GTCTCTG CTTCACTG GAG
.........ACTC G GATACACCCTTCTACTC
..............................CCTCCTGCTACCGATTAA
"^^PfTAAl
\
LMPGCDYSLFKDGIEPMWEDEKHKRGGRW ITL
NKQQRR5DL
_
MASARYK
uiwBsmr
© Q
Search for Primers & Probes
Search Options Subsearches
Search in: 3 + Strand 0 - Strand Search Mode: @ Select
^ Complex Substrate
© PGR Primers
Compatible with the Q Forward Primer   3 Reverse Primer
2 TaqMan Probes & PCR Pairs Compatible with the Q Upper Probe
O Lower Probe
G Molecular Beacons & PCR Pairs O Nested Primers O Sequencing Primers O Hybridization Probes
siRNA Probes
After successfull search show:   All Results
f   Search ^
Cancel j ■ Appiy
Parameters
Rang
es
Defaults ^)
MASARYK UMV9STTY
Search for Primers <& Probes
I
Search Options Subsearches
Search method: Compatible Pairs
0 Eliminate Ambiguous Bases
0 Duplex-free Oligonucleotides
^ Highly Specific Oligonucleotides (3'-end Stability)
□ S'-end Stability
□ siRNA Internal Stability
0 Oligonucleotides with CC Clamp
0 Oligonucleotides within Selected Tm Limits
2] Hairpin-free Oligonucleotides
Eliminate Mono- and Di-Nucleotide Repeats
Detect Sequence Repeats 0 Eliminate Frequent Oligonucleotides 25 Omit High Secondary Structure Regions in the Template 0 Check Primers/Probe Sequence Constraints 0 Restrict the Number of C Bases 5? Eliminate False Priming Oligonucleotides and Q Continue Above Search in Other File(s) [J Consensus Primers
(   Search )
Q   Cancel ^) Apply )
^ Parameters j Ranges ^)
C
Defaults
3
MASARYK UMVHBTTY
File: Human 4E.seq
PCR
		
		
		
Optimal Annealing Temperature: 50.8 °C (Max: 66.3 °Q
	Position and Length			cc M	P.E#	Score
Pi£du*----			78.9	29.6	n/a	697
Forward Primer	9LS	22	\ 56.9	45.5	47L/47L	S40
Reverse Primer	L753	2^	' 55.3	29.6	489 / 489	834
	--g7S-	24	56.5	33.3	479 / 479	9L7
Lower Oligo	1694	23	55.4	39. L	457 / 457	841
Product Tm - Reverse Primer Tm. Primers Tm difference: 1.6 °C		23.6	°C Comments:	
	Concentration			
Forward Primer	200.0	nM		
Reverse Primer	200.0	nM		
Upper Oligo	200.0	nM		
Lower Oligo	200.0	nM		
Monovalent Cation	SO.O	niM		
Free Mg[2+)	0.7	niM		
Total Na[ + ] Equivalent: 1SS.8 mM
34
MASARYK
UMVBtsmr
Tile: ERCA2 gene.seq
Selected Primers
AY436640:L543SF22	
5' CAATATATACCCTACTCCCCTA 3'	
Length:	22-mer
Score:	802 points
5' Position:	L5438
Tm/tm: 53.4	52.6 °C
AC/Ag (25 °Q: -30.5	-29.2 kcal/mol
AS/M: -472.1	-449.5 cal/°K*mol
AH/Ah: -L7L.3	-L63.2 kcal/mol
3'AC:	-6.5 kcal/mol
Degeneracy:	/-^1
P.E.#:	(443/443)
1/E:	4^53 nmol/A2G0
3L.L ^g/A2M	
AY436640:L59L7R20
5' CACCTACATATTAC C C C A C A 3'
Length:
Score:
3' Position:
AC/Ag (25 °C): A5/As: AH/Ah: 3'AC:
Degeneracy:
P.E.*:
1/E:
53.L -28.6 -430.5 -L57.0
20-mer 9L4 points L59L7
53.8 DC -28.5 kcal/mol -4L9.6 cal/üK*mol -153.6 kcal/mol -6.9 kcal/mol
sL 17^
15 nmol/A2G0 3L.0 M9/A2C0
Priming Efficiency PE Score
35
MASARYK
uiwBsrrv
Secondary structures ]
HAIRPIN intramolecular DIMER intermolecular
eoe	Current Oligo Duplexes	
File: BRCAZ gene.seq		
Current Oligo 2L-mer [5042]
[Currentt Oligo] - The most stable 3'-dinner: & of hydrogen bonds = L0: AC = -0.7 kcal/mol
5 1  GAArTAGArAAATTCAAArrA 3 1 III   II   II III
fCurrent- Oligo! - The most stable 3-dimer: #of hydrogen bonds = L0; AC = -73 kcal/mol; Tm = 2.9°C
5 h TAATTTGAftrrrATCTAftTTC 3 *
I I I I I I I I I I
31 G rrAATC TArrrAAU tttaat 51
The most stable dinier overall: & of hydrogen bonds = 10: AC = -7.4 kcal/mol: Tm = 2.2°C
51   GAATrAUATAAArrCAAATTA 31
Hairpin: loop ■ 5 nt: AC ■ -3.0 kcal/mol; Tm = 54.5 "^C
I I I I I A 31 ATTAAACTTAAAT
MA&ARYK UMVB8TTY
8 O 8
Current Oligo Hairpin Sterns
1
file: GRCA2 gene.seq
CurrentOligo 2L-nner [5042]
			
L # of paired bases = 5; loop = 5 nt; AG = -3.0 kcal/mol; Tm = 54.6 *C			
5042 GAA 1 1 1 5056 tTT	IT 5046 AA 5052	5 rGAATTAG-III A 3 'ATTAAACTTAAAT-1	
			
2. £ of paired bases = 6: loop = 5 nt; AG = 0.2 kcal			;mol:Tm = 2L7*C
5043 AATT 1 1 5061 TTAA	ACA 5049 1 1 ACT 5055	5 1 GAATTAGATA-, II       II A 3 1 ATTAAAC'ITA-1	
			
3. # of paired bases = 4; loop = 2 nt: AC = 0.9 kcal/mol; Tm = S/7 °C			
5052 Mil 1 1 506L TTI	7T 5055 1 ■lA 5059	5 1 GAATTAGATAAArrC-i 1 1 1 1 3 1AITAAA-1	
MASARYK UMVB8TTY
O O0   Reverse Primer False Priming Sites
Hie: M13MP18
Reverse Primer ML3MP18 63 L0R19 (positive strand) * Priming efficiency of the perfect match is 482 (above the threshold) *
Priming efficiency: 482 (above the threshold)
S'(6328)   GGTTTTCCCAGTC ACC ACG (6310)3'
I I I I I I I I I I I I I I I I I I I
3 (6328)  ccaaaagggtcagtgctgc (6310)5*
Priming efficiency: 244 (above the threshold)
51(6328)   GGTTTTCCCAGTCACGACG [63l0)3f
III   I I I I llllll
3' (626)  agcaaatggtc—tgctgc (610)5'
Priming efficiency: 193 (above the threshold)
S1(6328)   GGTTTTCCCAGTCACGACG (6310)3f
III    MINIM III
3(S12S)   t_ct_aagt_ggt_cagtg-tgc (5108)5r
in
38
MASARYK
uiwBsrrv
0 ^ O     Forward Primer Composition
Tile: BRCA2 gcrc.seq
Forward Primer AY43G640 6275F19
	64.2'	(nearest neighbor method]
Tm	56,5*	[nearest neighbor method]
Tm	70.8'	[%CC method]
Tm	56*	|2[A+TT + 4fC+Q# method)
	tv	[ttGC method]
Tm (DN A RNA)[ 1M Mai	74.7*	WGQ method)
	1.59	Isingle strand]
Molecular Weight	5-SK	[one strand)
Molecular Weight	11.7K	(two strands]
	47.4	[dsDNAJ
Base	Kumber&3t	
A	2	[iCS*]
C	5	[2G.3H]
G	4	[21.13«)
T	fi	142AM]
A + T	LO	[52-Sfc]
C + C	9	14 7.4ft]
39
MASARYK UMV9STTY
Oligonucleotide Database
file: Nev/Database.cdb
X			il				<8?	u		rB 1	# of Records: 29
□ 21
□ 22
□ 23 24
■_■ 25
□ 26 U 27 U 2S
Date
ID Number
12/02/06 12/02/06 L2/02/06 L2/02/06 L2/02/06 L2/02/06 L2/02/06 12/02/06
AY436640 AY436640 AY436640 AY436640 AY436640 AY436640 AY436640 AY436640
5916R19 S916R20 5937R21 5937R22 4695U22 5325U22 57S6L23 5S60LL9
Sequence
AATC C CTC C CTTTA CTCTC CAATGCCTGCCTCTAGTCTG TCAATTTCTTTA C CTTC C CAT TTC AATTTCTTTAC CTTGGCAT TCCCTTAA CAAAA CTAATCCAT A ATTA C CTCTTTCTTATC C C AA CTCTCCCTA CAA CATTATCACTC AACAACCAAACCCAACCTC
-Dhn.dG		P.E / p.e.		Tm /tm	
	sc	430	430	54.L	54.5
0.3	5C	366	450	SO.9	57.2
i-		J49	449	54.7	53. L
	aBaS	1:3	45S	55.9	53.3
0.3	sc	432	432	54.5	53.0
0.3	sc	453	453	53.3	53.0
-0.3	sc	451	45L	54.S	55.0
0.9		444	444	55.3	55.9
Oligonucleotide 5et& (64)
		Forward	Rever&e	Upper	Lower
	#	Primer	Primer	ON go	Qligo
		l	2		A
□	36	8	23	25	2S
□	42	S	24	25	2S
	47		L4	25	27 4
□	39	9	15	25	27
□	33	9	16	25	27
□	61	9	L7	25	27
□	4S	9	LS	25	27
Checked Set of nested primers
c
This database is linked to BRCA2 gene.seq
40
MASARYK UMVB8TTY
Restri
zyme Sites in Protein
Hie: BRCA2 gene.seq
#      EhZyme i£ilííu |;aDnD ^JfeDD fiSBB ^JOIID ^«DD ,^e.DD i^iDD j250DD ^SJDD ,Z5Ě.DD |25iD0 ^tODO   r i: í "V ^KiDO   r i: r-"i. ,
33 EcoRI I   I II II \^ ~\       I      TIP _I- I   I   TT I    f '
34
35
EcoRV EsP3l
36 Fsel
37 Fspl 3B Gsul
39 Hindlll
40 Hpal
41 Kpnl
42 Mlul
43 Munl
44 Nael
45 Narl
46 NcpI 47|Ndel
#	Enzyme	5ite	#Cuts	Positions & Fragment 5izes												
																
41	Kpnl	GT2VpzY6	S	-21253	23654	6S	23722	52	23774	237	24011	585	24596	162	24758	A
				629	253B7	1219	26606	22851								J
42	Mlul	TRLRVyA7	5	-22233	22674	2824	25498	576	26074	106	26180	244	26424	23033		
43	Munl	QL3Nawl5	L0	-212S7	23620	355	23975	351	24326	282	24608	242	24850	72	24922	
				551	25273	714	25987	187	26174	420	26594	22863				
44	Nael	AG2PAxR6	7	-21S23	230S4	597	23681	1286	24967	86	25055	573	25626	149	25775	
				623	26398	23059										
45	Narl	GA2APzR6	L	-20043	24S64	24593										
46	Ntol	PW3HGwMS	4	-2236L	22546	336	22S82	887	23769	531	24300	25157				
47	Ndel	HM2lawY5	2	-20366	24541	1211	25752	23705								
4S	Nhcl	AS2LAK-6	16	-22276	22631	322	22953	iss	23153	88	23226	27	25255	461	23714	
				369	240S3	312	24395	288	246S3	151	24834	273	25107	536	25643	
				402	26045	30	26075	210	26285	372	26657	22800				¥
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Search: 22454to27004 End Cut Type: Blunt, Odd, 5"-overhang, S'-overhang
MASARYK UMV9STTY
8 O O Hybridization Time
file: M13MP1S
DNA Length: [ Concentration:
21
nt.
200.0 nWi
L.29S Mg/mL
VÁ = 45.4 sec T   =3 min 47 sec
MASARYK
uiwBsmr
Concentrations
file: GRCA2 gene.seq
© Constant Concentration     (2r Constant Volume
© Current + Oligo: O Current -Oligo: 2 Entire Sequence (ds): O Forward Primer: 2 Reverse Primer: 0 PCR Product (ds): C Upper Oligo: C Lower Oligo:
5.OS nmol/ODr3Z.5 ug/OD 4.67 nmol/ODr30.9 ug/OD 0.00L nmol/ODr 4S.L ug/OD S.9S nmol/ODr 35.0 ug/OD 5.3L nmol/ODh34.0 ug/OD 0.146 nmol/DDr 4S.L ug/OD 4.S3 nmol/ODr31.2 ug/OD
4.67 nmol/ODr30.9 ug/OD
[ 32-5
MS
or
or
in
L.O OD(260)
5.0S4 nmol
50S.4 uL
yields
LO.O uM
MASARYK
uiwBsrrv
AHP2 cDNA (TAIR database)|
Sequence: AT3G29350.1 Date last modified   2007-04-17 Name   AT3G29350.1 Tail Accession   Sequence:4010737427 Sequence Length (bp) 82 7
1 ACAATTC GCG AGAAAGACAA AACACAAGTT TCTTCTTCTT GGGATTGGCT 51 ATTTCCAGAA ATCCAAGTCA ATAATCAAAG TCCAAACAAA AAAATCCTCT 101 CCCAATCTCC GCTTCACTCT TCTCATGGAC GCTCTCATTG CTCAGCTTCA 151 GAGACAATTT CGTGATTACA CCATTTCTCT CTACCAACAG GGGTTTTTGG 201 ATGATCAATT TACTGAGTTG AAAAAGCTAC AAGATGATGG AAGTCCTGAT 251 TTTGTGTCTG AAGTGCTTTC ACTTTTCTTT GAAGATTGTG TGAAGCTTAT 301 CAGTAACATG GCTAGAGCTT TGGACACGAC AGGAACTGTA GATTTTAGTC 351 AGGTAGGTGC TAGTGTGCAT CAATTGAAGG GTAGTAGCTC AAGTGTTGGT 401 GCCAAGAGGG TCAAAACTTT GTGTGTTAGC TTCAAGGAAT GTTGTGAAGC 451 TAAGAACTAC GAAGGGTGTG TGAGATGTTT GCAGCAAGTG GATATTGAGT 501 ACAAGGCGTT AAAGACAAAG CTTCAAGATA TGTTCAATCT TGAGAAACAG 551 ATCATTCAAG CTGGTGGTAT AGTTCCTCAA GTGGATATTA ACTAAAGAGA 601 CTAGTCCATA AGAAGAAAAA AG AT GATG AC TTTCTTTCTT TAGTTTCTCT 651 TCTAAATTAT TTTGGATTTG GTGTTTGCTC AAAAACTCAA TAAAATATGT 701 GCAAAAAGAA ACAAAAACAA GTGATGGTTG TTTATAAATC AGTAGTATGT 751 ATTGTTTGAT CTCATCCGAG AAAATTGAAA CCATTGGACT AATGAATGTG 801 ATGATAATAT ATATTGGTTT GCTTCTG
44
MASARYK
umvbwty
101 CCCAATCTCC GCTTCACTCT TCTCATGGAC GCTCTCATTG CTCAGCTTCA 151 GAGACAATTT CGTGATTACA CCATTTCTCT CTACCAACAG GGGTTTTTGG 201 ATGATCAATT TACTGAGTTG AAAAAGCTAC AAGATGATGG AAGTCCTGAT 251 TTTGTGTCTG AAGTGCTTTC ACTTTTCTTT GAAGATTGTG TGAAGCTTAT 301 CAGTAACATG GCTAGAGCTT TGGACACGAC AGGAACTGTA GATTTTAGTC 351 AGGTAGGTGC TAGTGTGCAT CAATTGAAGG GTAGTAGCTC AAGTGTTGGT 401 GCCAAGAGGG TCAAAACTTT GTGTGTTAGC TTCAAGGAAT GTTGTGAAGC 451 TAA GAACTAC GAAGGGTGTG TGAGATGTTT GCAGCAAGTG GATATTGAGT 501 ACAAGGCGTT AAAGACAAAG CTTCAAGATA TGTTCAATCT TGAGAAACAG 551 ATCATTCAAG CTGGTGGTAT AGTTCCTCAA GTGGATATTA ACT AAA GAGA
EcoRI restriction site
5'......GlAATTC......3
3"......CTTAAl G......5'
Design of primers
AHP2ex_up
y- CCG GAA TTC ATG GAG GCT CTC ATT GCT GAG - 3' AHP2ex_low
5'- CCG GAA TTC TTA GTT A AT ATC CAC TTG AGG - 3'
45
MASARYK
uiwBsrrv
101 CCCAATCTCC GCTTCACTCT TCTCgTCGgT GCTCTCTTTC C'l'CAqCTTCA 151 GAGACAATTT CGTGATTACA CCATTTCTCT CTACCAACAG GGGTTTTTGG 201 ATGATCAATT TACTGAGTTG AAAAAGCTAC AAGATGATGG AAGTCCTGAT 251 TTTGTGTCTG AAGTGCTTTC ACTTTTCTTT GAAGATTGTG TGAAGCTTAT 301 CAGTAACATG GCTAGAGCTT TGGACACGAC AGGAACTGTA GATTTTAGTC 351 AGGTAGGTGC TAGTGTGCAT CAATTGAAGG GTAGTAGCTC AAGTGTTGGT 401 GCCAAGAGGG TCAAAACTTT GTGTGTTAGC TTCAAGGAAT GTTGTGAAGC 451 TAAGAACTAC GAAGGGTGTG TGAGATGTTT GCAGCAAGTG GATATTGAGT 501 ACAAGGCGTT AAAGACAAAG CTTCAAGATA TGTTCAATCT TGAGAAACAG 551 ATCATTCAAG CTGGTGGTAT AGTTpiHT(JAA (.JTGGATATTA ACTA^AGAGA
EcoRI restriction site
5'......G| AATTC......3
3"......CTTAAl G......5
Design of primers
AHP2 ex_up
53- CCG GAA TTC ATG GAC GCT CTC ATT GCT CAG -AHP2ex_low
5'- CCG GAA TTC TTA GTT AAT ATC CAC TTG AGG - 33
MASARYK UMVB8TTY
LITERATURE
■ Artificial DNA: Methods and Applications; Khudyakov, Y.E., Fields, W.A., Ed. (2003)
■ PCR Primer: A Laboratory Manual (2003)
■ OLIGO Primer analysis software, Version 7
■ Expert Opin TherPat. 2014, 24(7):801-19. Oligonucleotide delivery: a patent review (2010 - 2013).
■ AAPS Journal 2009, 11(1): 195-203.
Targeted Delivery Systems for Oligonucleotide Therapeutics
■ Large-scale de novo DNA synthesis: technologies and applications Nature Methods 2014, 11 (5): 499
47
MA&ARYK UMV9STTY
Discovery is not in seeking new landscapes, but in having new eyes...
Marcel Proust
48