Thermostable type-A DNA polymerase mutants with increased polymerization rate and resistance to inhibitors

The invention claimed is: 1. A mutant thermostable Type-A DNA polymerase consisting of or comprising: a first mutation at residue 507 of wild-type Taq DNA polymerase, which has the sequence of SEQ ID NO:4, or at a residue corresponding to residue 507 of wild-type Taq DNA polymerase in another thermostable Type-A DNA polymerase; and at least one additional mutation at a residue selected from 59, 155, 245, 375, 508, 734, and 749 of wild-type Taq DNA polymerase, or at a corresponding residue in another thermostable Type-A DNA polymerase, wherein the combination of mutations provides a mutant polymerase that possesses a faster polymerization rate and a higher resistance to polymerization activity inhibitors than the wild-type DNA polymerase from which it is derived. 2. The mutant of claim 1 , wherein the mutant DNA polymerase is a mutant Taq DNA polymerase, which comprises an E507K mutation as the first mutation. 3. The mutant of claim 1 , which is a mutant Taq DNA polymerase and which comprises mutations at the following residues: G59, V155, L245, L375, E507, E734, and F749. 4. The mutant of claim 3 , which comprises the following mutations: G59W, V155A, L245M, L375V, E507K, E734G, and F749I. 5. The mutant of claim 1 , which is a mutant of a thermostable Type-A DNA polymerase other than Taq DNA polymerase and which comprises mutations at residues corresponding to the following residues of Taq DNA polymerase: G59, V155, L245, L375, E507, E734, and F749. 6. The mutant of claim 1 , which is a mutant Taq DNA polymerase and which comprises mutations at the following residues: G59, L245, L375, E507, K508, E734, and F749. 7. The mutant of claim 6 , which comprises the following mutations: G59W, L245M, L375V, E507K, K508R, E734G, and F749I. 8. The mutant of claim 1 , which is a mutant of a thermostable Type-A DNA polymerase other than Taq DNA polymerase and which comprises mutations at residues corresponding to the following residues of Taq DNA polymerase: G59, L245, L375, E507, K508, E734, and F749. 9. The mutant of claim 1 , which comprises mutations at the following residues of Taq DNA polymerase: L245, E507, and F749, or at corresponding residues in another thermostable Type-A DNA polymerase. 10. The mutant of claim 1 , which comprises mutations at the following residues of Taq DNA polymerase: L245, L375, E507, E734, and F749, or at corresponding residues in another thermostable Type-A DNA polymerase. 11. The mutant of claim 1 , consisting of or comprising the sequence of SEQ ID NO:12, SEQ ID NO:14, SEQ ID NO:16, SEQ ID NO:18, SEQ ID NO:20, SEQ ID NO:24, SEQ ID NO:26, SEQ ID NO:28, SEQ ID NO:30, SEQ ID NO:32, SEQ ID NO:34, SEQ ID NO:36, or SEQ ID NO:38, wherein the polymerase possesses a faster polymerization activity than wild-type Taq polymerase and is resistant to inhibitors of wild-type Taq polymerase. 12. A kit for amplification of a target nucleic acid, said kit comprising the mutant DNA polymerase of claim 1 and packaging materials therefor. 13. A method of polymerization of a target nucleic acid from a primer that specifically binds to the target nucleic acid, said method comprising: combining the primer with the target nucleic acid and the mutant thermostable Type-A DNA polymerase of claim 1 , wherein the mutant thermostable Type-A DNA polymerase consists of or comprises: a first mutation at residue 507 of wild-type Taq DNA polymerase or at a residue corresponding to residue 507 of wild-type Taq DNA polymerase in another thermostable Type-A DNA polymerase; and at least one additional mutation at a residue selected from 59, 155, 245, 375, 508, 734, and 749 of wild-type Taq DNA polymerase, or at a corresponding residue in another thermostable Type-A DNA polymerase, wherein the combination of mutations provides a mutant polymerase that possesses a faster polymerization rate and a higher resistance to polymerization activity inhibitors than the wild-type DNA polymerase from which it is derived, and providing conditions under which the polymerase extends the primer using the sequence of the target as a template for incorporation of nucleotides. 14. The method of claim 13 , which is a method of PCR. 15. The method of claim 14 , which is a method of fast PCR. 16. The method of claim 13 , wherein the conditions include the presence of an inhibitor of the wild-type DNA polymerase at a concentration that is inhibitory to the wild-type DNA polymerase. 17. The method of claim 13 , wherein the target nucleic acid is present in blood or a fraction of blood. 18. The method of claim 13 , wherein the target nucleic acid is present in plant material or a sample containing plant material.