The nucleotide sequence of gene 18 of bacteriophage T4 was determined by the Maxam-Gilbert method, partially aided by the dideoxy method. To confirm the deduced amino acid sequence of the tail sheath protein (gpl8) that is encoded by gene 18, gpl8 was extensively digested by trypsin or lysyl endopeptidase and subjected to reverse-phase high-performance liquid chromatography. Approximately 40 peptides, which cover 88% of the primary structure, were fractionated, the amino acid compositions were determined, and the corresponding sequences in DNA were identified. Furthermore, the amino acid sequences of 10 of the 40 peptides were determined by a gas phase protein sequencer, including N-and C-terminal sequences. Thus, the complete amino acid sequence of gp18, which consists of 658 amino acids with a molecular weight of 71,160, was determined. * Corresponding author. "Achromobacter lyticus" M467-1, was purchased from Wako Junyaku Co. Polynucleotide kinase and all of the restriction enzymes used were purchased from Takara Shuzo Co. Methanesulfonic acid (4 M) was purchased from Pierce Chemical Co., and all other reagents were analytical grade, from either Nakarai Chemicals or Wako Junyaku Co. Nutrient broth, tryptone, yeast extract, Bacto-Agar, and Casamino Acids were purchased from Difco Laboratories. Medium and buffer. M9A medium was used to grow E. coli. It contained, per liter of water, 6 g of Na2HPO4, 3 g of KH2PO4, 0.2 g of MgSO4. 7H20, 0.5 g of NaCl, 1 g of NH4C1, 4 g of glucose, and 10 g of Casamino Acids. Phages were stored in B+ buffer, which contained, per liter of water, 7 g of Na2HPO4, 4 g of NaCl, and 3 g of KH2PO4, supplemented with 1 mM MgSO4 for use. Phage, plasmids, and bacterial strains. T4D.23amH11 is from our collection. T4D.18am mutants (Fig. 1) were kindly supplied by W. B. Wood and J. King. E. coli BE was used as a nonpermissive host for amber mutant phages, and E. coli CR63 was the permissive host. E. coli JM103 was used to propagate M13 phages and to prepare replicative-form DNA of M13 phage. Three E. coli BE strains, which carry plasmids p662, p655, and p664, respectively, were kind gifts from Tom Mattson. Each of the three plasmids contains an EcoRI fragment which forms approximately one-third of gene 18 (Fig. 1). Marker rescue test. Marker rescue of T4D.18am mutants by plasmids was performed as described by Mattson et al. (21). The results are also shown in Fig. 1. DNA preparations for sequencing. DNA preparations for the Maxam-Gilbert method have been described by Christensen and Young (8). DNA was 5' end labeled with polynucleotide kinase, and the strands were then separated by polyacrylamide gel electrophoresis, or alternatively, the double-stranded DNA was cut with a restriction enzyme and the desired fragment was purified by polyacrylamide gel electrophoresis. DNA sequencing procedures. The Maxam-Gilbert method was done essentially as described by Maxam and Gilbert (22). The dideoxy method was carried out as described by Messing (23). Preparation of gpl8. Gpl8 was prepared as described ...
