Tzipora Goldkorn scite author profile

Proteolysis of cytochrome c with pepsin results in the rapid preferential cleavage of the peptide bond between residues 66 and 67. The resulting 1-66 heme peptide is biologically inactive, binds readily cyanide and carbon monoxide, is oxidized in air, but is not reduced by ascorbate. The spectrum of this heme peptide has the same maxima observed for shorter heme peptides, but the absorption coefficients of their maxima are significantly lower.

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A simple and efficient enzymatic method for covalent attachment of DNA to cellulose. Application for hybridization-restriction analysis and for in vitro synthesis of DNA probes

Goldkorn

Prockop

1986

Nucl Acids Res

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Single-stranded DNAs (ssDNAs) were covalently bound by a simple and efficient enzymatic method to a solid support matrix and used to develop several new procedures for gene analysis. The novel procedure to prepare a ssDNA stably coupled to a solid support employed T4 DNA ligase to link covalently oligo (dT)-cellulose and (dA)-tailed DNA. Beginning with essentially any double stranded DNA the procedure generates a ssDNA linked by its 5' end to a cellulose matrix in a concentration of over 500 ng per mg. DNA from the plasmid pBR322 (4300 bp) and a fragment of the beta-globin gene (1800 bp) were coupled to the solid support and used for several experiments. The ssDNAs on the cellulose efficiently hybridized with as little as 5 pg of complementary double-stranded DNAs. The DNA hybrids formed on the solid support were specifically and efficiently cleaved by restriction endonucleases. These specific restriction cuts were utilized for the diagnosis of correct sequences. In addition, the ssDNA on the solid support served as an efficient template for the synthesis of complementary ssDNAs. The complementary synthesized ssDNAs were uniformly labeled, more than two kilobases in size, and largely full length. About 85% of the ssDNA linked to cellulose was available for the synthesis of complementary DNA, and after strand-separation, the preparation was reusable for the synthesis of additional complementary DNA.

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Kinetic and spectroscopic evidence for different forms of ferric cytochrome c at very low ionic strength and neutral pH

Goldkorn¹,

Schejter²

1977

FEBS Letters

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