Mutans streptococci¿¡ ´ëÇÑ polyphosphateÀÇ Ç×±ÕÈ¿°ú
ANTIBACTERIAL EFFECT OF POLYPHOSPHATES ON MUTANS STREPTOCOCCI
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KMID : 0358920030300010080
Abstract
Ä¡¾Æ¿ì½ÄÁõÀÇ ¿øÀαÕÀÎ S. mufaus GS5¿Í S. sobrinus 6715¿¡ ´ëÇÑ polypÀÇ È¿°ú¸¦ °üÂûÇÏ¿© º¸´Ù ¾ÈÀüÇÏ°í È¿°úÀûÀÎ Ä¡¾Æ¿ì½ÄÁõ ¿¹¹æÀ» À§ÇÑ ÀÓ»óÀû¿ëÀÇ °¡´É¼ºÀ» °íÂûÇÏ°íÀÚ Ã¹Â°, ´Ù¾çÇÑ »ç½½±æÀÌÀÇ polyP¸¦ ÷°¡ÇÑ ÈÄ Èí±¤µµ¸¦ ÃøÁ¤ÇÏ¿© MIC¸¦ °áÁ¤ÇÏ°í, µÑ°, ½ÇÇè±ÕÁÖ¸¦ Èí±¤µµ 0.3~0.5±îÁö Áõ½Ä½ÃŲ ÈÄ MIC ³óµµÀÇ polyP¸¦ ÷°¡ÇÏ¿© Èí±¤µµÀÇ º¯È¸¦ ÃøÁ¤ÇÔÀ¸·Î½á ±ÕÁÖÁõ½Ä ÈÄ ¼ºÀå ¾ïÁ¦È¿°ú¸¦ °üÂûÇÏ¿´À¸¸ç, ¼Â°, »ý±Õ¼ö ÃøÁ¤À¸·Î potyPÀÇ Ç×±ÕÈ¿°ú¸¦ Æò°¡ÇÏ¿´°í, ³Ý°, ÇÙ»êÀ¯¸®ÀÇ Á¤µµ·Î polyPÀÇ Å³·¹ÀÌ¼Ç ÀÛ¿ë¿©ºÎ¸¦ °üÂûÇÏ¿´À¸¸ç, ´Ù¼¸Â°, polyPÀÇ ºñ¼ö¿ë¼º ±Û·çÄ ÇÕ¼º´É·ÂÀ» °üÂûÇÏ¿´À¸¸ç, ¿©¼¸Â°, Åõ°úÀüÀÚÇö¹Ì°æÀ¸·Î ¼¼Æ÷¸·°ú ¼¼Æ÷Áú ³»ÀÇ ±¸Á¶Àû º¯È¸¦ °üÂûÇÏ¿´´Ù. ÀÌ»óÀÇ ¿¬±¸¸¦ ÅëÇÏ¿©, polyPÀÇ »ì±ÕÀÛ¿ëÀÌ S. mutans¿Í S. sobrinus¿¡ ´ëÇÑ ¼ºÀåÀ» ¾ïÁ¦½ÃÅ°´Â È¿°ú°¡ ÀÖ´Â °ÍÀ¸·Î °¡´ÆµÈ´Ù. ÀÌ¿Í °°Àº ¼ºÀå ¾ïÁ¦È¿°ú´Â potyPÀÇ Å³·¹À̼ǿ¡ ÀÇÇÑ °ÍÀ̶ó±âº¸´Ù´Â ±ÕÁÖ ¼¼Æ÷ÀÇ ±¸Á¶Àû, ÇüÅÂÀû º¯È°¡ ÁÖµÈ ¿äÀÎÀ̾ú´ø °ÍÀ¸·Î ÆǴܵȴÙ.
Mutans streptococci, especially S. mutans and S. sobrinus strongly implicated in pathogenesis of dental caries, the major cause of tooth loss in children. Use of an antibacterial agent controlling dental caries has been rationalized. The present study was performed to observe the antibacterial effect of inorganic polyphosphates (polyP) on S. mutans and S. sobrinus. S. mutans GS5 and S. sobrinus 6715 were grown in brain-heart infusion broth with or without polyP. Minimal inhibitory concentration (MIC) of polyP for S. mutans GS5 was determined to be 0.08% and that for S. sobrius 6715 was 0.17%. PolyP 15 added to the growing culture of S. mutans GS5 and S. sobrinus 6715 at their exponential phase was as effective in inhibiting the growth of S. mutans GS5 and S. sobrinus 6715 as polyP added at the very beginning of the culture. More than 85% of the cells lost their viability determined by viable cell count when polyP 15 was added to the culture of growing S. mutans GS5 at MIC, suggesting that polyP 15 has bacterial effect on the bacterium. And more than 99.9% of the cells lost their viability determined by viable cell count when polyP 15 was added to the culture of growing S. sobrinus 6715 at MIC, suggesting that polyP 15 has bacterial effect on the bacterium. Intracellular nucleotide release from S. mutans GS5 and S. sobrinus 6715 was increased in the presence of polyP 15 for 5h but was not really reversed by the addition of divalent cations like Ca+¢¥ and Mg". The majority of the cells appeared to be atypical in their shape, demonstrating accumulation of highly electron-dense granules and ghost cells. The overall results suggest that polyP have a strong bactericidal activity against S. mutans and S. sobrinus in which lysis in relation to chelation may not play the major role but unknown mechanism that possibly affects the viability of the bacterium may be involved. PolyP may be used as an agent for prevention of dental caries.
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Ç×±ÕÈ¿°ú;Polyphosphate;S. mutans;S. sobrinus;Antibacterial
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