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促进DNA在体内向大鼠下颌下腺的转移及GRP-Ca基因调控。

Facilitated DNA transfer to rat submandibular gland in vivo and GRP-Ca gene regulation.

作者信息

O'Connell B C, Ten Hagen K G, Lazowski K W, Tabak L A, Baum B J

机构信息

Clinical Investigations and Patient Care Branch, National Institute of Dental Research, National Institutes of Health, Bethesda, Maryland 20892-1190, USA.

出版信息

Am J Physiol. 1995 Jun;268(6 Pt 1):G1074-8. doi: 10.1152/ajpgi.1995.268.6.G1074.

Abstract

The internalization of DNA can be facilitated by adenovirus infection. Using the replication-deficient adenovirus, Ad-dl312, and a plasmid-based firefly luciferase gene as a reporter, we have optimized the uptake and expression of DNA in rat submandibular glands in vivo. Luciferase expression is transient and peaked at approximately 18 h after infection. Luciferase activity increased with plasmid concentration and was greatest at 10(9) to 10(10) plaque-forming units of Ad-dl312 per gland. We next examined the expression in vivo of plasmids containing deletions of the glutamine/glutamic acid-rich protein (GRP-Ca isoform) gene upstream region linked to a chloramphenicol acetyltransferase (CAT) reporter. Constructs with 9.4, 6.3, and 2.7 kb and 17 base pairs of upstream sequence gave relative CAT activities of 100, 30, 7.6, and 38.5, respectively. With the 9.4-kb GRP-Ca construct, CAT was preferentially expressed in acinar cells, which is characteristic of GRP. This gene transfer approach should prove useful in the further study of gene expression in salivary glands and other organs.

摘要

腺病毒感染可促进DNA的内化。我们使用复制缺陷型腺病毒Ad-dl312和基于质粒的萤火虫荧光素酶基因作为报告基因,在体内优化了大鼠下颌下腺中DNA的摄取和表达。荧光素酶表达是短暂的,在感染后约18小时达到峰值。荧光素酶活性随质粒浓度增加而增加,在每腺10(9)至10(10)个Ad-dl312噬斑形成单位时最高。接下来,我们检测了含有与氯霉素乙酰转移酶(CAT)报告基因相连的富含谷氨酰胺/谷氨酸蛋白(GRP-Ca同工型)基因上游区域缺失的质粒在体内的表达。具有9.4、6.3和2.7 kb以及17个碱基对上游序列的构建体的相对CAT活性分别为100、30、7.6和38.5。使用9.4-kb GRP-Ca构建体时,CAT优先在腺泡细胞中表达,这是GRP的特征。这种基因转移方法在唾液腺和其他器官的基因表达进一步研究中应会证明是有用的。

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