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GS-Taq DNA Polymerase Set(dNTP mix Æ÷ÇÔ), cat.3017S/1,000U
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BEAMSBIO GS-Taq DNA Polymerase Set

GS-Taq DNA Polymerase (recombinant).  Store at –20¡É

#3017S
1,000 U

2 vials of 500 U/vial : 5 U/µl. Supplied with 1.0 ml of 10X GS-Taq Rxn Buffer and  0.5ml of 10mM dNTP mix


Features

l         Taq DNA Polymerase fortified with High Fidelity and 3¡¯à5¡¯ proofreading activity

l         Generates TA cloning site of PCR products.

l         PCR for difficult genomic DNA and PCR above 10KB viral DNA template

l         RT-PCR

Description

GS-Taq DNA polymerase is heat stable Taq DNA polymerase optimized for  PCR above10KB. This enzyme has an optimum temperature around 74¡É and can withstand temperatures up to 95¡É.  The enzyme has 3¡¯à5¡¯ proofreading activity with high fidelity. Our GS-Taq DNA polymerase is provided with x10 reaction buffer.  Our product has extremely high purity free from any nucleic acid contaminants and impurities,  which was purified through ion exchange column and affinity column chromatography.

Source

E. coli clone, recombinant gene from Thermus aquaticus YT1.

Concentration

5 U/µl.  Successful amplification can be achieved using 1~2U / 50§¡ reaction, typically for PCR target ~ 5 kb.  Further optimization, such as cycling time, reaction temperature, enzyme unit (2~4U/,50§¡), dNTP amount, and number of cycling, will be required for PCR target greater than 5~10kb.

Applications

l         PCR above 10KB viral DNA template and 5kb for genomic DNA

l         High throughput PCR and High reproducibility with 3¡¯à5¡¯ proofreading activity.

l         Generation of PCR products for TA cloning.

l         RT-PCR.

Quality Control

The BEAMSBIO GS-Tag DNA Polymerase is confirmed free of endodeoxyribonucleases, exodeoxyribonucleases and ribonucleases by strict quality tests, which shows satisfactory PCR results above 10 kb with viral DNA templates and up to 5 kb with genomic DNA templates.

Definition of Activity Unit

One unit is defined as the amount of enzyme required to catalyze the incorporation of 10nmol of dNTPs into an acid-insoluble product in 30 minutes at 74¡É.

STANDARD UNIT ASSAY CONDITIONS 

50mM Tris-HCl (pH9.0 at 25¡É), 50mM NaCl, 10mM MgCl2, 200¥ìM dATP, dCTP, dGTP, and radiolabeled dTTP, and 12.5¥ìg activated calf thymus DNA in a 50¥ìl reaction.

Storage Buffer

50mM Tris-HCl (pH8.0), 100mM NaCl, 0.1mM EDTA, 2mM DTT, 1.0% Triton X-100 and 50% glycerol.  Store at -20¡É.

10X  Reaction Buffer

100mM Tris-HCl (pH8.3 at 25¡É), 500mM KCl and 15mM MgCl2. Buffer is optimized for use with 0.2mM for each of dNTPs.

Inhibition and Inactivation

Inactivated by phenol/chloroform extraction.  Heat denaturation is not possible.

BEAMSBIO GS-Taq DNA Polymerase Set ¸Å´º¾ó

PCR Protocol using GS-aq DNA Polymerase

1. Prepare PCR tubes for the experimental samples to be amplified.
ÁõÆøÇÒ ½ÇÇè½Ã·á¿¡ ÀûÇÕÇÑ PCRÆ©ºê¸¦ ÁغñÇÑ´Ù.

2. Add the components in order according to following recipe :
´ÙÀ½ ¼ººÐÇ¥¸¦ ÂüÁ¶ÇÏ¿© ½ÇÇè¿ë Àç·á¸¦ ¼ø¼­´ë·Î ³Ö´Â´Ù.

  Distilled water,                                                      36~43
§¡ * (balance to total vol. 50§¡)
  x10 Reaction buffer,                        5
§¡
  10mM dNTP mix,                                              1~3
§¡
  GS-Taq DNA Polymerase,                                    0.5~1
§¡ (5U/§¡) (ÅõÀÔ ÈÄ °¡º±°Ô ¼¯´Â´Ù)

  DNA templates(10~200ng/
§¡),                     0.2~1§¡
  Primer, forward(10pmol/
§¡),                             0.2~2§¡
  Primer, backward(10pmol/
§¡),                           0.2~2§¡
-----------------------------------------------------------------------------
                                                                 total  50
§¡
 * Primers(template
¿Í ¹Ì¸® ¹èÇÕ »ç¿ë°¡´É)¸¦ ¸¶Áö¸·¿¡ ³Ö´Â °ÍÀÌ ÁÁ´Ù.

3. Mix gently and rapidly. Centrifuge down PCR tubes immediately after mixing.
°¡º±°í ½Å¼ÓÇÏ°Ô ¼¯°í, Áï½Ã ª°Ô ¿ø½ÉºÐ¸®ÇÏ¿© ¹ÝÀÀ¹°À» ¾Æ·¡·Î ¸ðÀº´Ù.

4. Perform PCR using optimized cycling conditions.  Suggested cycling parameters for PCR using PCR Master Mix are :
´ÙÀ½ ¿îÀüÁ¶°ÇÀ» ÂüÁ¶ÇÏ¿© PCR Master Mix ÃÖÀû PCR¿îÀüÁ¶°ÇÀ» ¼³Á¤ÇÏ¿© ½ÇÇèÀ» ¼öÇàÇÑ´Ù.

  - Step 1 :  initial denaturation,                                     94~95
¡É for 45sec.
  - Step 2 :  denaturation,                                    94
¡É for 45sec.
            annealing,                                    Tm-5
¡É for 45sec.
            extension,                                    68~72
¡É for 0.5~1 min/kb
           * 25~30 cycles recommended
           * 10KB
³»¿ÜÀÎ °æ¿ì, 10~15 ½ÎÀÌŬ ¼öÇàÈÄ 20~30Ãʾ¿ ½Ã°£À»
             
´Ã¸®¸é¼­ 15~20 ½ÎÀÌŬ Ãß°¡·Î ¼öÇàÇÔ(Á¶°Ç ÃÖÀûÈ­ ÇÊ¿ä).
  - Step 3 :  final extension,                                    72
¡É for 7~20min.

5. Cool down below 15¡É until harvest.

PCR Troubleshooting

1. PCR band°¡ ÀüÇô ¾ø´Â °æ¿ì :
- ¹ÝÀÀ¹° ¼ººÐ ¹èÇÕ¿¡ Âø¿À°¡ ¾ø´ÂÁö È®ÀÎÇÑ´Ù.  ¼ººÐ´©¶ô ¿©ºÎ ?
- PCR
¿îÀüÁ¶°ÇÀÌ ÀûÇÕÇÏ¿´´ÂÁö È®ÀÎÇÑ´Ù.  PCR¹ÝÀÀ±â ¿îÀü ½Ç¼ö ¿©ºÎ ?
- PCR Master Mix
¿ëµµ¿¡ ¸ÂÁö ¾Ê´Â DNA template ÁõÆø½Ãµµ ¿©ºÎ ?
 Long PCR Master Mix, Pfu PCR Master Mix
µî ÀûÇÕÇÑ PCR System ¼±ÅÃ
- Primer Design
ÀûÇÕ, Template DNA ¼Õ»ó, Inhibitor ÀÜÁ¸ ¿©ºÎ µî °ËÅä

2. PCR band°¡ »Ñ¿¸°Ô ¢ßºö½º¹ÙÀÌ¿À¿¡¼­ ÆǸÅÇÑ ¹ÙÀÌ¿À¼ÒÀç Á¦Ç°ÀÇ Ç°Áú ºÒ¸¸¿¡ ´ëÇÏ¿© °ø±ÞÀÚ¸¦ ÅëÇÏ¿© ´ç»ç¿Í ¹Ì¸® ÇùÀÇ°¡ ¿Ï·áµÈ °æ¿ì º°µµÀÇ ºñ¿ë ºÎ´ã¾øÀÌ Á¦Ç°À» ±³È¯ÇÏ¿© µå¸³´Ï´Ù. µû¶ó¼­, Ç°Áú ºÒ¸¸¿¡ ´ëÇÏ¿© ¹Ì¸® ÇùÀÇ°¡ ÀÌ·ç¾îÁö±â Àü±îÁö´Â ¹°Ç°À» ÀÓÀÇ·Î ¹Ý¼ÛÇÏ¿©¼­´Â ¾ÈµÇ¸ç, ÀÌ °æ¿ì ¹ß»ýÇÏ´Â ¸ðµç ºñ¿ëÀº °í°´ÀÌ ºÎ´ãÇÏ¿©¾ß ÇÕ´Ï´Ù. ¹ÙÀÌ¿À ¼ÒÀç Á¦Ç°Àº ¿î¼Û ½Ã Ç°ÁúÀÌ º¯µ¿µÉ ¼ÒÁö°¡ Å©±â ¶§¹®¿¡ Á¦Ç° Ç°Áú ¹®Á¦´Â ´ë°³ ¿î¼Û µµÁß¿¡ ¹ß»ýÇÕ´Ï´Ù´ç»ç¿¡¼­´Â ¹Ý¼ÛµÈ ¹°Ç°À» °Ë»ç ÈÄ °Ë»ç °á°ú¿¡ »ó°ü¾øÀÌ Áï½Ã Æó±âÇÕ´Ï´Ù.

A return authorization is required before shipping.  Please do not return any product without first contacting Beams Biotechnology or distributor for a return authorization.  All return authorizations must be issued directly from Beams Biotechnology.  In the case of a purchasing error, it is our policy to deny return of product.  Due to the temperature sensitivity of the products, we are unable to resell returned goods, as we are not assured of the quality.






 
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