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Christoph J. Hueck Michael J. Hantman Vivek Bajaj Christine Johnston Catherine A. Lee Samuel I. Miller 《Molecular microbiology》1995,18(3):479-490
Salmonella typhimurium secreted proteins (Ssp) were previously implicated in epithelial cell invasion. Here we describe four genes ( sspB , sspC , sspD , and sspA ), located between spaT and prgH , which encode proteins of 63, 42, 36, and 87 kDa, respectively. These Ssp are homologous to Shigella flexneri secreted proteins lpaB, lpaC, lpaD and lpaA. A non-invasive mutant with a transposon insertion in sspC lacks Ssp of 87,42 and 36 kDa. Complementation analyses show that sspC and sspD encode the 42 and the 36 kDa Ssp, while the 87 kDa Ssp is encoded by sspA . sspC and sspD , but not sspA are required for invasion. Amino-terminal sequencing shows that SspC and SspA are secreted without amino-terminal processing. We further demonstrate that Ssp secretion requires proteins encoded by prgHIJK , homologous to the Shigella lpa secretion system, since SspA is abundantly secreted by wild-type bacteria but is completely retained within the cellular fraction of a prgHIJK mutant. A precipitate containing abundant SspC and three other major Ssp of 63,59 and 22 kDa was isolated from culture supernatants of wild-type bacteria. These data indicate that major secreted invasion determinants of S. typhimurium are structurally and functionally homolgous to S. flexneri lpa proteins. 相似文献
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Londo Thomas R. Kehoe Terry Kates Steven A. Hantman Susan Gordon Neal F. 《International journal of peptide research and therapeutics》1998,5(4):285-297
Methods for peptide assembly consist of techniques that allow for construction of complex sequences. The advantage of solid-phase methodologies is automation of the repetitive processes of deprotecting, washing, and coupling protected amino acids (acylation). However, for difficult sequences the crude product contains a variety of side products that must be removed to provide the desired target peptide in sufficient concentration and purity. This paper illustrates that high efficiency purification method-development can be achieved by combining purification and analysis on a single platform. Incorporation of fast LC-based assays using polystyrene-based POROS® Perfusion Chromatography media permitted rapid overall processing times from crude peptide purification through fraction pooling and product verification. Application of these technologies to the purification of peptides at scales of 100 mg is demonstrated. 相似文献
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Between Powhatan and Quirank: Reconstructing Monacan Culture and History in the Context of Jamestown
One of the more enigmatic events in the history of European colonization in the New World is the generally tolerant reception the Jamestown colonists received in 1607 from Powhatan, the paramount chief of the Powhatan people of Tidewater Virginia. Understanding that event requires an anthropological study of the complex sociopolitical relations between the coastal Powhatan and the less-well-known interior cultures of the native world. This article is primarily concerned with describing one such interior culture, the Monacan, a people who ethnohistoric texts suggest were less complex than, and a principal enemy of, the Powhatan. Analysis of those texts, and insights derived from archeology, provide a picture of the Monacan that leads to a different perspective on the context of the Jamestown settlement, and on relations of power between indigenous cultures in the precontact world. 相似文献
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Thomas R. Londo Terry Kehoe Steven A. Kates Susan Hantman Neal F. Gordon 《Letters in Peptide Science》1998,5(4):285-297
Methods for peptide assembly consist of techniques that allow for construction of complex sequences. The advantage of solid-phase methodologies is automation of the repetitive processes of deprotecting, washing, and coupling protected amino acids (acylation). However, for difficult sequences the crude product contains a variety of side products that must be removed to provide the desired target peptide in sufficient concentration and purity. This paper illustrates that high efficiency purification method-development can be achieved by combining purification and analysis on a single platform. Incorporation of fast LC-based assays using polystyrene-based POROS® Perfusion Chromatography media permitted rapid overall processing times from crude peptide purification through fraction pooling and product verification. Application of these technologies to the purification of peptides at scales of 100 mg is demonstrated. 相似文献
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Joshua Dacre Matt Colligan Thomas Clarke Julian J. Ammer Julia Schiemann Victor Chamosa-Pino Federico Claudi J. Alex Harston Constantinos Eleftheriou Janelle M.P. Pakan Cheng-Chiu Huang Adam W. Hantman Nathalie L. Rochefort Ian Duguid 《Neuron》2021,109(14):2326-2338.e8
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