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Home > Learning center > Recombinant Protein Purification > ´Ù¾çÇÑ ½ÇÇè Àû¿ë »ç·Ê > ºÐºñÇü ´Ü¹éÁúÀÇ ½±°í ºü¸¥ Á¤Á¦

ºÐºñÇü ´Ü¹éÁúÀÇ ½±°í ºü¸¥ Á¤Á¦

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ºÐºñÇü his-tagged proteinÀÇ °£´ÜÇÑ Á¤Á¦

Capturem¢â His-Tagged Purification Maxiprep Kit


¡á Introduction
»ý¹°ÇÐÀû È°µ¿¿¡ ÇÊ¿äÇÑ post-translational modificationÀÌ ÁøÇàµÇ¸ç Á¤È®ÇÏ°Ô folding µÇ°í Á¶¸³µÈ ÃæºÐÇÑ ¾çÀÇ ÀçÁ¶ÇÕ ´Ü¹éÁúÀ» ¹ßÇöÇÏ°í Á¤Á¦ÇÏ´Â °ÍÀº »ý¹°ÇÐÀû ºÐ¼®ÀÇ ÁÖ¿ä °úÁ¦ÀÌ´Ù. ÇÑ °¡Áö °¡´É¼º ³ôÀº ÇØ°áÃ¥Àº ÀÌ·¯ÇÑ ´Ü¹éÁú ºÐÀÚ¸¦ Æ÷À¯µ¿¹° ¼¼Æ÷¿¡¼­ ºÐºñÇü ´Ü¹éÁú·Î °ú¹ßÇöÇÏ´Â °ÍÀε¥, ÀÌ´Â È¿¸ð ¶Ç´Â baculovirus ½Ã½ºÅÛº¸´Ù Á¤È®ÇÑ folding°ú º¯ÇüÀ¸·Î È°¼º ´Ü¹éÁúÀ» »ý»êÇÏ´Â µ¥ ´õ È¿°úÀûÀÌ´Ù (Dalton and Barton 2014). ¹ßÇö½ÃŲ ´Ü¹éÁúÀÌ ¼¼Æ÷ ¹è¾ç ¹èÁö·Î ºÐºñµÇ¸é ¼¼Æ÷°¡ °è¼Ó ¼ºÀåÇÔ¿¡ µû¶ó ¹è¾ç »óÃþ¾×À» ±³Ã¼ÇØÁָ鼭 ¿©·¯ ¹ø ´Ü¹éÁúÀ» ȸ¼öÇÒ ¼ö ÀÖÀ¸¹Ç·Î ¸¹Àº ¾çÀÇ ´Ü¹éÁúÀ» ¾òÀ» ¼ö ÀÖ´Ù. ¶ÇÇÑ ¼¼Æ÷¸¦ ¿ëÇØÇÏ´Â ´ë½Å ¹è¾ç ¹èÁö¿¡¼­ ´Ü¹éÁúÀ» Á¤Á¦Çϸé, ¼¼Æ÷ ¾È¿¡ Á¸ÀçÇÏ´Â ´Ü¹éÁú ºÐÇØÈ¿¼Ò¿¡ ´ëÇÑ ³ëÃâÀ» ÁÙ¿© ¼Õ»óµÇÁö ¾ÊÀº È°¼º ´Ü¹éÁúÀÇ ¼öÀ²À» ³ôÀÏ ¼ö ÀÖ´Ù.

±âÁ¸ÀÇ ÀçÁ¶ÇÕ his-tagged ´Ü¹éÁú Á¤Á¦ ¹æ¹ýÀº IMAC (Immobilized Metal Affinity Chromatography) Ä÷³ÀÌ ÇÊ¿äÇÏ°í, Ä÷³À» ·ÎµùÇϱâ Àü¿¡ Å»¿° ¹× ¹öÆÛ ±³È¯ µî ±ä ÀýÂ÷¿Í ¼ö¸¹Àº Ä÷³ ¼¼Ã´ °úÁ¤ÀÌ ÇÊ¿äÇÏ´Ù.
¹Ý¸é, Capturem¢â His-Tagged Purification Maxiprep Kit´Â »õ·Î¿î °í¿ë·® ¸âºê·¹ÀÎÀÌ ÀÖ´Â maxi spin columnÀ» »ç¿ëÇϹǷΠÀÌ·¯ÇÑ ¹ø°Å·Î¿î ¸¹Àº °úÁ¤À» »ý·«ÇÒ ¼ö ÀÖ¾î, °£´ÜÈ÷ 15ºÐ º¥Ä¡Å¾ °úÁ¤À¸·Î 2.5 §·ÀÇ his-tagged ´Ü¹éÁúÀ» Á¤Á¦ÇÒ ¼ö ÀÖ´Ù. ºÐºñÇü ´Ü¹éÁúÀ» Æ÷ÇÔÇÏ´Â ¹èÁö´Â BSA Á¦°Å, Å»¿° ¶Ç´Â ¹öÆÛ ±³È¯ ¾øÀÌ Capturem membrane¿¡ Á÷Á¢ ·ÎµåÇÒ ¼ö ÀÖ´Ù. Capturem ÇÁ·ÎÅäÄÝ¿¡ »ç¿ëµÇ´Â ÀûÀº elution º¼·ýÀº ´Ü¹éÁúÀ» °íµµ·Î ³óÃà½Ãų ¼ö ÀÖÀ¸¹Ç·Î, ´ëºÎºÐÀÇ °æ¿ì ¿øÇÏ´Â ¹öÆÛ¿¡ Èñ¼®ÇÒ ¼ö Àֱ⠶§¹®¿¡ º°µµÀÇ ¹öÆÛ ±³È¯ÀÌ ºÒÇÊ¿äÇÏ´Ù.

¡á Results
Purification of active protein from culture supernatants
Capturem his-tagged Á¤Á¦ ½Ã½ºÅÛÀ» Å×½ºÆ®Çϱâ À§ÇØ bicistronic IRES vector¸¦ »ç¿ëÇÏ¿© 293T cell¿¡¼­ ºÐºñ ´Ü¹éÁú (6xhis-tagged Metridia luciferase)°ú Çü±¤ transfection control (DsRed-Express2)À» °°ÀÌ ¹ßÇöÇÏ°í Metridia luciferase È¿¼ÒÀÇ Á¤Á¦ Àü°ú ÈÄ È°¼ºÀ» ÃøÁ¤ÇÏ¿´´Ù. Metridia luciferase´Â ¼¼Æ÷ ³»¿¡¼­ À¯ÁöµÇ´Â ´Ù¸¥ luciferase¿Í ´Þ¸® ºÐºñ ´Ü¹éÁúÀ̱⠶§¹®¿¡ Å×½ºÆ® »ùÇ÷Π¼±ÅÃÇÏ¿´À¸¸ç, ´Ù¸¥ luciferase¿Í ¸¶Âù°¡Áö·Î È°¼ºÀ» luminometer·Î ÃøÁ¤Çϱ⠽¬¿î ÀåÁ¡ÀÌ ÀÖ´Ù. ¶ÇÇÑ µ¿ÀÏÇÑ RNA Àü»çü¿¡¼­ µÎ °³ÀÇ °³º° À¯ÀüÀÚ¸¦ µ¿½Ã¿¡ ¹ßÇöÇÒ ¼ö ÀÖ´Â bicistronic IRES vector¸¦ »ç¿ëÇÏ¿©, Çü±¤ Çö¹Ì°æ (±×¸², ÆгΠA)À¸·Î DsRed-Express2 reporter¸¦ È®ÀÎÇÏ¿´°í, À̸¦ ÅëÇØ »ùÇà Á¤Á¦ Àü¿¡ 6xhis-tagged Metridia luciferase°¡ Àß ¹ßÇöµÇ¾ú´Â Áö È®ÀÎÇÒ ¼ö ÀÖ¾ú´Ù.
Transfection 48½Ã°£ ÈÄ, ¼¼Æ÷ ¹è¾ç »óÃþ¾×À» ¿ø½ÉºÐ¸®ÇÏ¿© ¸ðµç debris¸¦ Á¦°ÅÇÑ ÈÄ Capturem His-Tagged Purification Maxiprep Kit¸¦ »ç¿ëÇÏ¿© ¼¼Æ÷¹è¾ç »óÃþ¾×À¸·ÎºÎÅÍ his-tagged Metridia luciferase¸¦ ¾Æ·¡¿Í °°ÀÌ Á¤Á¦ÇÏ¿´´Ù. Luciferase È°¼ºÀ» Á¤Á¦ °úÁ¤ÀÇ ¿©·¯ ´Ü°è¿¡¼­ ÃøÁ¤ÇÏ¿´°í (±×¸², ÆгÎB) ´Ü¹éÁúÀÌ È¿°úÀûÀ¸·Î ³óÃàµÈ °ÍÀ¸·Î ³ªÅ¸³µÀ¸¸ç, º» Á¦Ç°À» »ç¿ëÇÑ Á¤Á¦ Á¶°ÇÀÌ luciferase È°¼º¿¡ ¿µÇâÀ» ÁÖÁö ¾ÊÀ½À» È®ÀÎÇÏ¿´´Ù.


±×¸². Capturem¢â His-Tagged Purification Maxiprep Kit¸¦ »ç¿ëÇÏ¿© Á¤Á¦ÇÑ his-tagged Metridial luciferaseÀÇ ³ôÀº ¼öÀ² ¹× È°¼º
ÆгΠA. 293T ¼¼Æ÷¿¡¼­ Metridia luciferase ¹ßÇö È®ÀÎ
6xhis-tagged Metridia luciferase¿Í Àû»ö Çü±¤ ¸®Æ÷Å͸¦ °øµ¿ ¹ßÇöÇÏ´Â pEF1a-Metluc-6xHis-IRES2-DsRed-Express2 ¹ßÇö º¤Å͸¦ In-Fusion¢ç Cloning°ú pEF1alpha-IRES-DsRed-Express2 Vector¸¦ »ç¿ëÇÏ¿© Á¦ÀÛÇÏ¿´°í, Xfect Transfection ½Ã¾àÀ» »ç¿ëÇÏ¿© 293T ¼¼Æ÷¿¡ transfection ½ÃÄ×´Ù. ÀÌÈÄ DsRed-Express2 ¸®Æ÷Å͸¦ »ç¿ëÇÏ¿© transfection È¿À²À» ¸ð´ÏÅ͸µÇÏ¿´´Ù.
ÆгΠB. Á¤Á¦ Àü°ú ÈÄÀÇ Metridia luciferase ¼öÀ² ¹× È°¼º
His-tagged Metridia luciferase¸¦ ¹ßÇöÇÏ´Â 293T ¼¼Æ÷¿¡¼­ ¾òÀº ¹è¾ç »óÃþ¾×À» ÀÌ¿ëÇÑ Á¤Á¦ °úÁ¤ÀÇ ´Ü°è¸¶´Ù luciferase È°¼ºÀ» ÃøÁ¤ÇÏ¿´À¸¸ç, ÃÖÁ¾ elutionÇÑ »ùÇÿ¡¼­ ³ôÀº È°¼ºÀ» À¯ÁöÇÏ°í ÀÖÀ½À» È®ÀÎÇÏ¿´´Ù.

¡á Conclusions
Capturem¢â His-Tagged Purification Maxiprep Kit¸¦ »ç¿ëÇϸé 15ºÐ ¾È¿¡ BSA Á¦°Å, Å»¿° ¶Ç´Â buffer ±³È¯¾øÀÌ ¼¼Æ÷ ¹è¾ç »óÃþ¾×¿¡¼­ È°¼ºÀ» °¡Áö´Â ºÐºñÇü 6xhis-tagged ´Ü¹éÁúÀ» Á¤Á¦ÇÒ ¼ö ÀÖ´Ù. ±âÁ¸ ¹æ¹ý¿¡´Â ¸¹Àº ½Ã°£°ú ³ë·ÂÀÌ ÇÊ¿äÇßÁö¸¸ ÀÌÁ¦, Capturem¢â His-Tagged Purification ½Ã¸®Á ÀÌ¿ëÇÏ¸é º¸´Ù ½±°í ºü¸£°Ô ´Ü¹éÁúÀ» Á¤Á¦ÇÒ ¼ö ÀÖ´Ù.

¡á Method

Clarify 10 ml of cell culture supernatant (from a 10-cm dish) by centrifugation.

Equilibrate the column with 6 ml of xTractor Buffer.

Centrifuge the clarified sample through an equilibrated Capturem Maxiprep Nickel column.

Wash the column once with 6 ml of Wash Buffer.

Elute the secreted protein with 1 ml of Elution Buffer.

References  
Dalton, A. C. & Barton, W. A. Over-expression of secreted proteins from mammalian cell lines. Protein Sci. 23, 517-525 (2014).

¡á °ü·ÃÁ¦Ç°

Code

Á¦Ç°¸í

¿ë·®

635710

Capturem¢â His-Tagged Purification Miniprep kit

20 ȸ

635713

Capturem¢â His-Tagged Purification Maxiprep Kit

6 ȸ

635715 ¿Ü

Capturem¢â His-Tagged Purification Maxiprep Columns

25 columns

635724

Capturem¢â His-Tagged Purification Large Volume

4 ȸ

635714

Capturem¢â His-Tagged Purification 96-Well Plate

1 plate

635730

Capturem¢â His-Tagged Purification 24-Well Plate

1 plate

635656 ¿Ü

xTractor Buffer

100 §¢

635623

xTractor Buffer Kit (lysozyme, DNase I Æ÷ÇÔ)

1 set

635672 ¿Ü

ProteoGuard EDTA-Free Protease Inhibitor Cocktail

100 §¡

- His-tag À¶ÇÕ ´Ü¹éÁú Á¤Á¦ ¼±Åð¡À̵堺¸·¯°¡±â