Jasper Zu Putlitz, Stefan Wieland‡, Hubert E. Blum‡, Jack R. Wands

Slides:

Advertisements

Similar presentations

Date of download: 5/30/2016 From: Chronic Hepatitis B Virus Infection: Treatment Strategies for the Next Millennium Ann Intern Med. 2000;132(9):

Advertisements

Volume 118, Issue 1, Pages (January 2000)

Volume 16, Issue 3, Pages (March 2008)

Volume 130, Issue 3, Pages (March 2006)

Volume 148, Issue 2, Pages e7 (February 2015)

Volume 131, Issue 3, Pages (September 2006)

Jasper Zu Putlitz*, Stefan Wieland‡, Hubert E. Blum‡, Jack R. Wands*

Volume 44, Issue 2, Pages (February 2006)

Volume 141, Issue 2, Pages e3 (August 2011)

Volume 65, Issue 4, Pages (October 2016)

A Combinatorial CRISPR-Cas9 Attack on HIV-1 DNA Extinguishes All Infectious Provirus in Infected T Cell Cultures Gang Wang, Na Zhao, Ben Berkhout, Atze.

Self-Excising Retroviral Vectors Encoding the Cre Recombinase Overcome Cre- Mediated Cellular Toxicity Daniel P. Silver, David M. Livingston Molecular.

Molecular diagnosis of viral hepatitis

Volume 141, Issue 3, Pages (September 2011)

Volume 130, Issue 3, Pages (March 2006)

The homeodomain protein Cdx2 regulates lactase gene promoter activity during enterocyte differentiation Rixun Fang, Nilda A. Santiago, Lynne C. Olds,

Volume 124, Issue 7, Pages (June 2003)

Volume 148, Issue 2, Pages e7 (February 2015)

Volume 125, Issue 1, Pages 9-18 (July 2003)

Marco Baralle, Tibor Pastor, Erica Bussani, Franco Pagani

Mechanisms of HBV-related hepatocarcinogenesis

Volume 44, Issue 4, Pages (April 2006)

How viral genetic variants and genotypes influence disease and treatment outcome of chronic hepatitis B. Time for an individualised approach? Neil Rajoriya,

Volume 118, Issue 1, Pages (January 2000)

Hepatitis delta virus facilitates the selection of hepatitis B virus mutants in vivo and functionally impacts on their replicative capacity in vitro

Volume 2, Issue 4, Pages (October 2000)

Transcriptional activation of transforming growth factor-β1 in mesangial cell culture by high glucose concentration Brenda B. Hoffman, Kumar Sharma,

Sustained Inhibition of HBV Replication In Vivo after Systemic Injection of AAVs Encoding Artificial Antiviral Primary MicroRNAs Mohube Betty Maepa,

Volume 127, Issue 5, Pages (November 2004)

Volume 44, Issue 5, Pages (May 2006)

Complete Cure of Persistent Virus Infections by Antiviral siRNAs

Volume 10, Issue 1, Pages (July 2004)

Exon Circularization Requires Canonical Splice Signals

Volume 115, Issue 4, Pages (October 1998)

Volume 114, Issue 6, Pages (June 1998)

Ahmad S. Abdulkarim, Hong Cao, Bing Huang, Mark A. McNiven

Volume 13, Issue 2, Pages (February 2006)

Volume 68, Issue 4, Pages (April 2018)

Timothy M. Block, Ju-Tao Guo Gastroenterology

Volume 39, Issue 5, Pages (November 2003)

Targeting Hepatitis B Virus With CRISPR/Cas9

Inhibition of Retroviral Pathogenesis by RNA Interference

Rapid identification of efficient target cleavage sites using a hammerhead ribozyme library in an iterative manner Wei-Hua Pan, Ping Xin, Vuong Bui,

Andrew J Henderson, Ruth I Connor, Kathryn L Calame Immunity

Phosphorylation of Serine 2 within the RNA Polymerase II C-Terminal Domain Couples Transcription and 3′ End Processing Seong Hoon Ahn, Minkyu Kim, Stephen.

Yugong Ho, Felice Elefant, Stephen A. Liebhaber, Nancy E. Cooke

Volume 42, Issue 6, Pages (June 2005)

Volume 37, Issue 1, Pages (January 2010)

Volume 62, Issue 3, Pages (September 2002)

H. Randolph Byers, Mina Yaar, Mark S. Eller, Nicole L

Volume 42, Issue 3, Pages (March 2005)

Volume 133, Issue 4, Pages (October 2007)

Volume 132, Issue 4, Pages (April 2007)

Zongliang Gao, Elena Herrera-Carrillo, Ben Berkhout

Frpo: A Novel Single-Stranded DNA Promoter for Transcription and for Primer RNA Synthesis of DNA Replication Hisao Masai, Ken-ichi Arai Cell Volume.

Volume 128, Issue 3, Pages (March 2005)

Volume 116, Issue 3, Pages (March 1999)

Volume 8, Issue 4, Pages (October 2001)

Volume 127, Issue 4, Pages (October 2004)

Inclusion of jaagsiekte sheep retrovirus proviral elements markedly increases lentivirus vector pseudotyping efficiency Patrick L. Sinn, Erin R. Burnight,

Volume 4, Issue 1, Pages (January 1996)

RNA Polymerase II Activity of Type 3 Pol III Promoters

Volume 42, Issue 2, Pages (February 2005)

Cheryl A. Carlson, Dmitry M. Shayakhmetov, André Lieber

Promoting in Tandem: The Promoter for Telomere Transposon HeT-A and Implications for the Evolution of Retroviral LTRs O.N Danilevskaya, I.R Arkhipova,

Volume 22, Issue 2, Pages (February 2014)

Molecular Therapy - Nucleic Acids

Cell-surface expression of CD4 reduces HIV-1 infectivity by blocking Env incorporation in a Nef- and Vpu-inhibitable manner Juan Lama, Aram Mangasarian,

Volume 4, Issue 1, Pages (January 1996)

PML influences HBV transcription, expression, and replication through the HBV basal core promoter. PML influences HBV transcription, expression, and replication.

Presentation transcript:

Antisense RNA complementary to hepatitis B virus specifically inhibits viral replication Jasper Zu Putlitz*, Stefan Wieland‡, Hubert E. Blum‡, Jack R. Wands* Gastroenterology Volume 115, Issue 3, Pages 702-713 (September 1998) DOI: 10.1016/S0016-5085(98)70150-7 Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 1 Map of the HBV genome and location of antisense and sense RNAs used in the study. HBV has a 3.2-kb partially double-stranded DNA genome (central circle) from which four major classes of transcripts (circular, thin arrows) are synthesized. The 3.5-kb RNA contains coding regions (wide circular arrows) for the nucleocapsid (C) and the reverse transcriptase (pol). A subclass of this transcript with a slightly longer 5' end codes for the precore (pre-C) protein that, after processing, is secreted as HBeAg. The 2.4-kb RNA encompasses the preS1 open reading frame, which encodes for the large surface protein. The 2.1-kb RNA encompasses the preS2 and S open reading frames, which encode for the middle and small surface proteins, respectively. The smallest transcript (≈0.8 kb) codes for the X protein. The outermost arrows represent antisense RNAs AS 1, 2, 3, 4, and 5 (counterclockwise) as well as their sense RNA counterparts (clockwise). The table shows exact positions and lengths of antisense and sense RNAs on the genome of HBV, subtype adw2.16 ϵ, 5'-encapsidation signal on pregenomic RNA. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 2 Inhibition of HBV replication by antisense RNA. Southern blot analysis of nucleocapsid-associated replication products of HBV after cotransfection of a replication-competent HBV-HTD with antisense or sense RNA expression constructs. (A) No impact of antisense RNAs AS 1 (lane 1), AS 2 (lane 5), AS 3 (lane 9), and their sense counterparts (S 1, lane 2; S 2, lane 6; and S 3, lane 10) on HBV replication (respective wild-type replication levels are shown in lanes 3, 7, and 11) is observed. (B) A 60% inhibitory effect of antisense RNA AS 4 (lane 1) on HBV replication is detected compared with the wild-type replication level (lane 2). A 75% inhibitory effect of antisense RNA AS 5 (lane 4) but not sense RNA S 5 (lane 5) on HBV replication (compare with the respective wild-type level in lane 6) is observed. These experiments were repeated four times with similar results. NC, negative controls (mock-transfected HuH-7 HCC cells); DS, position of double-stranded linear HBV DNA. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 2 Inhibition of HBV replication by antisense RNA. Southern blot analysis of nucleocapsid-associated replication products of HBV after cotransfection of a replication-competent HBV-HTD with antisense or sense RNA expression constructs. (A) No impact of antisense RNAs AS 1 (lane 1), AS 2 (lane 5), AS 3 (lane 9), and their sense counterparts (S 1, lane 2; S 2, lane 6; and S 3, lane 10) on HBV replication (respective wild-type replication levels are shown in lanes 3, 7, and 11) is observed. (B) A 60% inhibitory effect of antisense RNA AS 4 (lane 1) on HBV replication is detected compared with the wild-type replication level (lane 2). A 75% inhibitory effect of antisense RNA AS 5 (lane 4) but not sense RNA S 5 (lane 5) on HBV replication (compare with the respective wild-type level in lane 6) is observed. These experiments were repeated four times with similar results. NC, negative controls (mock-transfected HuH-7 HCC cells); DS, position of double-stranded linear HBV DNA. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 3 Effect of antisense RNAs on HBsAg (left) and HBeAg (right) secretion. Cell culture supernatants after cotransfection of a replication-competent HBV-HTD with antisense or sense RNA expression constructs were assayed by radioimmunoassay for HBsAg or HBeAg. AS 4 and AS 5 substantially inhibit HBsAg and HBeAg secretion, whereas the sense RNA control S 5 does not. No effect on HBsAg secretion is noted for antisense RNAs AS 1, AS 2, and AS 3 as well as their sense RNA counterparts. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 4 Effect of antisense RNA species on DHBV replication and effect of transcriptionally silent antisense constructs on HBV replication. (A) Southern blot analysis of nucleocapsid-associated replication products of DHBV after cotransfection of a replication-competent DHBV-HTD with antisense or sense RNA expression constructs directed against HBV into LMH chicken HCC cells. The expression levels of HBV antisense RNAs in LMH cells were comparable with levels observed in HuH-7 cells (data not shown). No inhibitory effect of HBV antisense RNA AS 4 (lane 1) on DHBV replication is observed compared with the wild-type replication level (lane 2). No inhibitory effect of HBV antisense RNA AS 5 (lane 4) or sense RNA S 5 (lane 5) is detected compared with the wild-type replication level (lane 6). (B) Transcriptionally silent antisense constructs AS/S4 (lane 1) and AS/S5 (lane 4) do not inhibit HBV replication (respective wild-type replication levels are shown in lane 2 and lane 5). These experiments were repeated three times with similar results. NC, negative controls (mock-transfected HuH-7 HCC cells); DS, position of double-stranded linear DHBV- (A) or HBV- (B) DNA. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 5 (A) Detection of HBV antisense and sense transcripts. Northern blot analysis of total cellular RNA and detection of antisense and sense transcripts 3 days after transfection of respective expression constructs. Transcripts corresponding to AS 1 (lane 1), S 1 (lane 2), AS 2 (lane 3), S 2 (lane 4), AS 3 (lane 5), S 3 (lane 6), AS 4 (lane 7), AS 5 (lane 9), and S 5 (lane 10) are expressed at high levels in transfected cells. Note that the sense control RNA S 4 is not detectable. These experiments were repeated several times with similar results. Numbers below the lanes refer to the nt length of HBV sequences present in the transcripts. (B) Effect of antisense RNA on HBV transcript levels. Northern blot analysis of total cellular RNA and detection of HBV-associated as well as antisense- and sense-transcripts 3 days after cotransfection of a replication-competent HBV-HTD with antisense or sense RNA expression constructs. The signal at 3.5 kb corresponds to terminally redundant HBV transcripts of which a subpopulation is encapsidated into the nucleocapsid; signals at 2.4/2.1 kb correspond to the preS1 and preS2/S transcripts, respectively. Coexpression of antisense RNAs AS 4 (lane 1) and AS 5 (lane 3) as well as sense RNA S 5 (lane 4) with HBV transcripts is observed. In the presence of antisense or sense RNAs, there is no significant reduction of the level of either the 3.5-kb or the 2.4/2.1-kb HBV transcripts detectable (compare lane 1 with lane 2; lanes 3 and 4 with lane 5). These studies were repeated three times with similar results. NC, negative control (mock-transfected HuH-7 HCC cells). Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 5 (A) Detection of HBV antisense and sense transcripts. Northern blot analysis of total cellular RNA and detection of antisense and sense transcripts 3 days after transfection of respective expression constructs. Transcripts corresponding to AS 1 (lane 1), S 1 (lane 2), AS 2 (lane 3), S 2 (lane 4), AS 3 (lane 5), S 3 (lane 6), AS 4 (lane 7), AS 5 (lane 9), and S 5 (lane 10) are expressed at high levels in transfected cells. Note that the sense control RNA S 4 is not detectable. These experiments were repeated several times with similar results. Numbers below the lanes refer to the nt length of HBV sequences present in the transcripts. (B) Effect of antisense RNA on HBV transcript levels. Northern blot analysis of total cellular RNA and detection of HBV-associated as well as antisense- and sense-transcripts 3 days after cotransfection of a replication-competent HBV-HTD with antisense or sense RNA expression constructs. The signal at 3.5 kb corresponds to terminally redundant HBV transcripts of which a subpopulation is encapsidated into the nucleocapsid; signals at 2.4/2.1 kb correspond to the preS1 and preS2/S transcripts, respectively. Coexpression of antisense RNAs AS 4 (lane 1) and AS 5 (lane 3) as well as sense RNA S 5 (lane 4) with HBV transcripts is observed. In the presence of antisense or sense RNAs, there is no significant reduction of the level of either the 3.5-kb or the 2.4/2.1-kb HBV transcripts detectable (compare lane 1 with lane 2; lanes 3 and 4 with lane 5). These studies were repeated three times with similar results. NC, negative control (mock-transfected HuH-7 HCC cells). Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions

Fig. 6 Antisense RNA AS 5 reduces the levels of encapsidated pregenomic RNA. Cotransfection of a replication-competent HBV-HTD with antisense RNA expression constructs AS 4 or AS 5 and control sense RNA S 5 into HuH-7 HCC cells. Nucleocapsids were isolated by ultracentrifugation through a sucrose cushion. (A) Primer extension analysis of encapsidated, pregenomic RNA from nucleocapsids. Relative amounts of encapsidated RNA were calculated using densitometric data after transfection efficiencies (shown at the bottom) were determined with an HGH assay as described in Materials and Methods. Note that encapsidated pregenomic RNA becomes undetectable (*) when antisense RNA AS 5 is present (lane 2), whereas the presence of antisense RNA AS 4 (lane 1, 110% of wild-type) does not reduce the amount of pregenomic RNA. A slight reduction (81% of the wild-type level) is noted in the presence of control sense RNA S 5 (lane 3). (B) Parallel quantification of nucleocapsids (p21) by immunoblot with an HBcAg-specific antiserum. Relative amounts of nucleocapsids were calculated using densitometric data after determination of transfection efficiencies with the HGH assay. No reductions in the level of nucleocapsids are observed for antisense RNAs AS 4 (lane 1) and AS 5 (lane 2) as well as for control sense RNA S 5 (lane 3) compared with the wild-type level (lane 4). These experiments were performed three times with similar results. Gastroenterology 1998 115, 702-713DOI: (10.1016/S0016-5085(98)70150-7) Copyright © 1998 American Gastroenterological Association Terms and Conditions