Inflammation Scan Using $^{99m}Tc-HMPAO$ Labelled Leukocytes

$^{99m}Tc-HMPAO$를 이용한 자가백혈구표지 및 그를 이용한 염증병소의 스캔

  • Yang, Woo-Jin (Department of Radiology, Catholic University Medicine College) ;
  • Chung, Soo-Kyo (Department of Radiology, Catholic University Medicine College) ;
  • Shinn, Kyung-Sub (Department of Radiology, Catholic University Medicine College) ;
  • Bahk, Yong-Whee (Department of Radiology, Catholic University Medicine College) ;
  • Kim, Hoon-Kyo (Department of Internal Medicine, Catholic University Medicine College)
  • 양우진 (가톨릭대학 의학부 방사선과학교실) ;
  • 정수교 (가톨릭대학 의학부 방사선과학교실) ;
  • 신경섭 (가톨릭대학 의학부 방사선과학교실) ;
  • 박용휘 (가톨릭대학 의학부 방사선과학교실) ;
  • 김훈교 (가톨릭대학 의학부 내과학교실)
  • Published : 1989.11.13

Abstract

Inflammation scan using radiolabelled leukocytes has high sensitivity and specificity. Several methods for labelling leukocytes have been evaluated using P-32 diisopropyl fluorophosphate (DFP-32), H-3 thymidine, Cr-51 chromate, Ga-67 citrate and Tc-99m-sulfur colloid. In-111-oxine has proved so far to be the most reliable agent for labelling leukocytes. In-111-oxine is, however, expensive, not easily available when needed, and its radiation dose to leukocytes is relatively high. Moreover, resolution of the resultant image is relatively poor. Tc-99m is still the agent of choice because of, as compared with the indium, its favorable physical characteristics, lower cost and availability. Now the technique for labelling the leukocytes with technetium is successfully obtained using the lipophilic HAPAO with higher efficiency for granulocytes than for other cells. With this technique it is possible to label leukocytes in plasma to improve the viability of the leukocytes. Inflammation scan using Tc-99m-HMPAO has been evaluated in several laboratories, and difference in methods for separation and labelling accounts for difference in efficiency, viability and biodistribution of the labelled leukocytes. We performed inflammation scan using leukocytes labelled with Tc-99m-HMPAO in three dogs 24 hours after inoculation of live E. Coli and A. Aureus in their right abdominal wall. We separated mixed leukocytes by simple sedimentation using 6% hetastarch (HES) and labelled the leukocytes with Tc-99m-HMPAO in 20% cell free plama diluted with phosphate buffer solution(Fig. 1). Uptake was high in the liver and spleen but is was minimal in the lungs on whole body scan. Kidneys and intestine showed minimal activity although it was high in the urinary bladder(Fig. 2). Uptake of labelled leukocytes in the inflammation site was do(mite on 2 hour-postinjection scan and abscess was clearly delineated on 24 hour-delayed scan with high target-to-nontarget ratio(Fig. 3, 4). Inflammation scan using mixed leukocytes labelled with Tc-99m-HMPAO is very sensitive and specific in early detection of inflammation.

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