Restriction Enzymes: PaeI (SphI)

Restriction Enzymes

Modifying Enzymes

PCR, qPCR, RT-PCR & dNTPs

Molecular Cloning

Nucleic Acid Purification

Molecular Labeling & Detection

In vitro Transcription

Electrophoresis Products

Nucleotides

Transfection Reagents

Reagents

PaeI (SphI)
Available in FastDigest® format
5'-G C A T G^C-3'
3'-C^G T A C G-5' 
digested lambda DNA
0.7% agarose
#ER0601
Supplied with:
10X Buffer B
10X Buffer Tango™ 500 u

1 ml
1 ml

#ER0602
Supplied with:
10X Buffer B
10X Buffer Tango™ 2500 u

1 ml
1 ml

Commercial Isoschizomers: BbuI, SphI

Related Documents (in pdf, ~55 KB):

Certificate of Analysis: #ER0601, #ER0602
MSDS (English)
MSDS (English-USA)
MSDS (German)
Chart (in pdf, 721 KB)
Brochure (in pdf, 316 KB)
Concentration
10 u/µl

Conditions for 100% Activity

Recommended
buffer Incubation
temperature Units for
overnight
incubation,
u/µg DNA Thermal
inactivation,
in 20 min
Enzyme activity, %

B
(blue) G
(green) O
(orange) R
(red) Tango™
(yellow)

1X 1X 1X 1X 1X 2X

Buffer B 37°C 0.1 65°C 100 50-100 0-20 0-20 50-100 0-20

Storage Buffer
10 mM potassium-phosphate (pH 7.0 at 25°C), 50 mM KCl, 1 mM DTT, 0.1 mM EDTA, 0.15% Triton X-100, 0.5 mg/ml BSA and 50% glycerol.

Ligation and Recleavage
After 50-fold overdigestion with PaeI, more than 95% of the digested DNA fragments can be ligated and recut.

Methylation Effects

Dam:
Dcm:
CpG:
EcoKI:
EcoBI: never overlaps
never overlaps
may overlap
never overlaps
may overlap - no effect.
- no effect.
- no effect.
- no effect.
- blocked.

Digestion of Agarose-embedded DNA
Minimum 5 units of the enzyme are required for complete digestion of 1 µg of agarose-embedded lambda DNA in 16 hours.

Compatible Ends
Hin1II, XceI.

Double Digestions using Tango™ Buffer, DoubleDigest™

Optimal
buffer
Enzyme activity, %

Tango™
(yellow)

1X 2X

Buffer B 50-100 NR

NR: buffer is not recommended, since enzyme activity is less than 20%.

Number of Recognition Sites in DNA Molecules

Lambda PhiX174 M13mp18/19 pBR322 pUC18/19 pUC57 pTZ19R/U pBluescriptIIKS(-/+) pBluescriptIISK(-/+) pACYC177 pACYC184

6 0 1 1 1 1 1 0 0 0 1

Lambda	PhiX174	M13mp18/19	pBR322	pUC18/19	pUC57	pTZ19R/U	pBluescriptIIKS(-/+)	pBluescriptIISK(-/+)	pACYC177	pACYC184
6	0	1	1	1	1	1	0	0	0	1

See also General Properties of Restriction Enzymes:

Updated baland�io 22, 2008 11:41

5'-G C A T G^C-3' 3'-C^G T A C G-5'		digested lambda DNA 0.7% agarose

#ER0601 Supplied with: 10X Buffer B 10X Buffer Tango™	500 u 1 ml 1 ml
#ER0602 Supplied with: 10X Buffer B 10X Buffer Tango™	2500 u 1 ml 1 ml
Commercial Isoschizomers: BbuI, SphI
Related Documents (in pdf, ~55 KB): Certificate of Analysis: #ER0601, #ER0602 MSDS (English) MSDS (English-USA) MSDS (German) Chart (in pdf, 721 KB) Brochure (in pdf, 316 KB)

Methylation Effects
Dam: Dcm: CpG: EcoKI: EcoBI:	never overlaps never overlaps may overlap never overlaps may overlap	- no effect. - no effect. - no effect. - no effect. - blocked.

Recommended buffer	Incubation temperature	Units for overnight incubation, u/µg DNA	Thermal inactivation, in 20 min	Enzyme activity, %
				B (blue)	G (green)	O (orange)	R (red)	Tango™ (yellow)
				1X	1X	1X	1X	1X	2X
Buffer B	37°C	0.1	65°C	100	50-100	0-20	0-20	50-100	0-20

Optimal buffer	Enzyme activity, %
	Tango™ (yellow)
	1X	2X
Buffer B	50-100	NR

PaeI (SphI) Available in FastDigest® format

PaeI (SphI)
Available in FastDigest® format