The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization

J. J. O'Leary; G. Browne; R. J. Landers; M. Crowley; I. Bailey Healy; J. T. Street; A. M. Pollock; J. Murphy; M. I. Johnson; F. A. Lewis; O. Mohamdee; C. Cullinane; C. T. Doyle

doi:10.1007/BF00157767

The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization

J. J. O'Leary
, G. Browne
, R. J. Landers
, M. Crowley
, I. Bailey Healy
, J. T. Street
, A. M. Pollock
, J. Murphy
, M. I. Johnson
, F. A. Lewis
, O. Mohamdee
, C. Cullinane
, C. T. Doyle

APC Microbiome Ireland

Research output: Contribution to journal › Article › peer-review

Abstract

Conventional solution-phase polymerase chain reaction (PCR) and in situ PCR/PCR in situ hybridization are powerful tools for retrospective analysis of fixed paraffin wax-embedded material. Amplification failure using these techniques is now encountered in some centres using archival fixed tissues. Such {black left-pointing small triangle}ailures' may not only be due to absent target DNA sequences in the tissues, but may be a direct effect of the type of fixative, fixation time and/or fixation temperature used. The type of nucleic acid extraction procedure applied will also influence amplification results. This is particularly true with in situ PCR/PCR in situ hybridization. To examine these effects in solution-phase PCR, β-globin gene was amplified in 100 mg pieces of tonsillar tissue fixed in Formal saline, 10% formalin, neutral buffered formaldehyde, Carnoy's, Bouin's, buffered formaldehyde sublimate, Zenker's, Helly's and glutaraldehyde at 0 to 4°C, room temperature and 37°C fixation temperatures and for fixation periods of 6, 24, 48 and 72 hours and 1 week. DNA extraction procedures used were simple boiling and 5 days' proteinase K digestion at 37°C. Amplified product was visible primarily yet variably from tissue fixed in neutral buffered formaldehyde and Carnoy's, whereas fixation in mercuric chloride-based fixatives produced consistently negative results. Room temperature and 37°C fixation temperature appeared most conducive to yielding amplifiable DNA template. Fixation times of 24 and 48 hours in neutral buffered formaldehyde and Carnoy's again favoured amplification. Fixed SiHa cells (containing 1-2 copies of HPV 16) were examined using PCR in situ hybridization for the amplification of HPV 16. Discrete and diffuse amplification signals were obtained. Neutral buffered formaldehyde fixation for 12-24 hours yielded amplifiable material suitable for use with PCR in situ hybridization. Overall amplification success within cellular preparations was 40%, with non-specific background staining also seen. Possible technical problems encountered with PCR in situ hybridization are discussed.

Original language	English
Pages (from-to)	337-346
Number of pages	10
Journal	Journal of Molecular Histology
Volume	26
Issue number	4
DOIs	https://doi.org/10.1007/BF00157767
Publication status	Published - Apr 1994

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10.1007/BF00157767

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O'Leary, J. J., Browne, G., Landers, R. J., Crowley, M., Healy, I. B., Street, J. T., Pollock, A. M., Murphy, J., Johnson, M. I., Lewis, F. A., Mohamdee, O., Cullinane, C., & Doyle, C. T. (1994). The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization. Journal of Molecular Histology, 26(4), 337-346. https://doi.org/10.1007/BF00157767

@article{0dc6d74ed3b4455c8b19c1f8fc120451,

title = "The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization",

abstract = "Conventional solution-phase polymerase chain reaction (PCR) and in situ PCR/PCR in situ hybridization are powerful tools for retrospective analysis of fixed paraffin wax-embedded material. Amplification failure using these techniques is now encountered in some centres using archival fixed tissues. Such \{black left-pointing small triangle\}ailures' may not only be due to absent target DNA sequences in the tissues, but may be a direct effect of the type of fixative, fixation time and/or fixation temperature used. The type of nucleic acid extraction procedure applied will also influence amplification results. This is particularly true with in situ PCR/PCR in situ hybridization. To examine these effects in solution-phase PCR, β-globin gene was amplified in 100 mg pieces of tonsillar tissue fixed in Formal saline, 10\% formalin, neutral buffered formaldehyde, Carnoy's, Bouin's, buffered formaldehyde sublimate, Zenker's, Helly's and glutaraldehyde at 0 to 4°C, room temperature and 37°C fixation temperatures and for fixation periods of 6, 24, 48 and 72 hours and 1 week. DNA extraction procedures used were simple boiling and 5 days' proteinase K digestion at 37°C. Amplified product was visible primarily yet variably from tissue fixed in neutral buffered formaldehyde and Carnoy's, whereas fixation in mercuric chloride-based fixatives produced consistently negative results. Room temperature and 37°C fixation temperature appeared most conducive to yielding amplifiable DNA template. Fixation times of 24 and 48 hours in neutral buffered formaldehyde and Carnoy's again favoured amplification. Fixed SiHa cells (containing 1-2 copies of HPV 16) were examined using PCR in situ hybridization for the amplification of HPV 16. Discrete and diffuse amplification signals were obtained. Neutral buffered formaldehyde fixation for 12-24 hours yielded amplifiable material suitable for use with PCR in situ hybridization. Overall amplification success within cellular preparations was 40\%, with non-specific background staining also seen. Possible technical problems encountered with PCR in situ hybridization are discussed.",

author = "O'Leary, \{J. J.\} and G. Browne and Landers, \{R. J.\} and M. Crowley and Healy, \{I. Bailey\} and Street, \{J. T.\} and Pollock, \{A. M.\} and J. Murphy and Johnson, \{M. I.\} and Lewis, \{F. A.\} and O. Mohamdee and C. Cullinane and Doyle, \{C. T.\}",

year = "1994",

month = apr,

doi = "10.1007/BF00157767",

language = "English",

volume = "26",

pages = "337--346",

journal = "Journal of Molecular Histology",

issn = "0018-2214",

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O'Leary, JJ, Browne, G, Landers, RJ, Crowley, M, Healy, IB, Street, JT, Pollock, AM, Murphy, J, Johnson, MI, Lewis, FA, Mohamdee, O, Cullinane, C & Doyle, CT 1994, 'The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization', Journal of Molecular Histology, vol. 26, no. 4, pp. 337-346. https://doi.org/10.1007/BF00157767

TY - JOUR

T1 - The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization

AU - O'Leary, J. J.

AU - Browne, G.

AU - Landers, R. J.

AU - Crowley, M.

AU - Healy, I. Bailey

AU - Street, J. T.

AU - Pollock, A. M.

AU - Murphy, J.

AU - Johnson, M. I.

AU - Lewis, F. A.

AU - Mohamdee, O.

AU - Cullinane, C.

AU - Doyle, C. T.

PY - 1994/4

Y1 - 1994/4

N2 - Conventional solution-phase polymerase chain reaction (PCR) and in situ PCR/PCR in situ hybridization are powerful tools for retrospective analysis of fixed paraffin wax-embedded material. Amplification failure using these techniques is now encountered in some centres using archival fixed tissues. Such {black left-pointing small triangle}ailures' may not only be due to absent target DNA sequences in the tissues, but may be a direct effect of the type of fixative, fixation time and/or fixation temperature used. The type of nucleic acid extraction procedure applied will also influence amplification results. This is particularly true with in situ PCR/PCR in situ hybridization. To examine these effects in solution-phase PCR, β-globin gene was amplified in 100 mg pieces of tonsillar tissue fixed in Formal saline, 10% formalin, neutral buffered formaldehyde, Carnoy's, Bouin's, buffered formaldehyde sublimate, Zenker's, Helly's and glutaraldehyde at 0 to 4°C, room temperature and 37°C fixation temperatures and for fixation periods of 6, 24, 48 and 72 hours and 1 week. DNA extraction procedures used were simple boiling and 5 days' proteinase K digestion at 37°C. Amplified product was visible primarily yet variably from tissue fixed in neutral buffered formaldehyde and Carnoy's, whereas fixation in mercuric chloride-based fixatives produced consistently negative results. Room temperature and 37°C fixation temperature appeared most conducive to yielding amplifiable DNA template. Fixation times of 24 and 48 hours in neutral buffered formaldehyde and Carnoy's again favoured amplification. Fixed SiHa cells (containing 1-2 copies of HPV 16) were examined using PCR in situ hybridization for the amplification of HPV 16. Discrete and diffuse amplification signals were obtained. Neutral buffered formaldehyde fixation for 12-24 hours yielded amplifiable material suitable for use with PCR in situ hybridization. Overall amplification success within cellular preparations was 40%, with non-specific background staining also seen. Possible technical problems encountered with PCR in situ hybridization are discussed.

AB - Conventional solution-phase polymerase chain reaction (PCR) and in situ PCR/PCR in situ hybridization are powerful tools for retrospective analysis of fixed paraffin wax-embedded material. Amplification failure using these techniques is now encountered in some centres using archival fixed tissues. Such {black left-pointing small triangle}ailures' may not only be due to absent target DNA sequences in the tissues, but may be a direct effect of the type of fixative, fixation time and/or fixation temperature used. The type of nucleic acid extraction procedure applied will also influence amplification results. This is particularly true with in situ PCR/PCR in situ hybridization. To examine these effects in solution-phase PCR, β-globin gene was amplified in 100 mg pieces of tonsillar tissue fixed in Formal saline, 10% formalin, neutral buffered formaldehyde, Carnoy's, Bouin's, buffered formaldehyde sublimate, Zenker's, Helly's and glutaraldehyde at 0 to 4°C, room temperature and 37°C fixation temperatures and for fixation periods of 6, 24, 48 and 72 hours and 1 week. DNA extraction procedures used were simple boiling and 5 days' proteinase K digestion at 37°C. Amplified product was visible primarily yet variably from tissue fixed in neutral buffered formaldehyde and Carnoy's, whereas fixation in mercuric chloride-based fixatives produced consistently negative results. Room temperature and 37°C fixation temperature appeared most conducive to yielding amplifiable DNA template. Fixation times of 24 and 48 hours in neutral buffered formaldehyde and Carnoy's again favoured amplification. Fixed SiHa cells (containing 1-2 copies of HPV 16) were examined using PCR in situ hybridization for the amplification of HPV 16. Discrete and diffuse amplification signals were obtained. Neutral buffered formaldehyde fixation for 12-24 hours yielded amplifiable material suitable for use with PCR in situ hybridization. Overall amplification success within cellular preparations was 40%, with non-specific background staining also seen. Possible technical problems encountered with PCR in situ hybridization are discussed.

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U2 - 10.1007/BF00157767

DO - 10.1007/BF00157767

M3 - Article

C2 - 8040006

AN - SCOPUS:0028196587

SN - 0018-2214

VL - 26

SP - 337

EP - 346

JO - Journal of Molecular Histology

JF - Journal of Molecular Histology

IS - 4

ER -

The importance of fixation procedures on DNA template and its suitability for solution-phase polymerase chain reaction and PCR in situ hybridization

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